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Using quantitative methods to understand leaf epidermal development

Published online by Cambridge University Press:  09 December 2022

Chi Kuan
Affiliation:
Institute of Plant and Microbial Biology, Academia Sinica, Taipei City, Taiwan
Shao-Li Yang
Affiliation:
Institute of Plant and Microbial Biology, Academia Sinica, Taipei City, Taiwan
Chin-Min Kimmy Ho*
Affiliation:
Institute of Plant and Microbial Biology, Academia Sinica, Taipei City, Taiwan
*
Author for correspondence: C.-M. K. Ho, E-mail: chmho@gate.sinica.edu.tw

Abstract

As the interface between plants and the environment, the leaf epidermis provides the first layer of protection against drought, ultraviolet light, and pathogen attack. This cell layer comprises highly coordinated and specialised cells such as stomata, pavement cells and trichomes. While much has been learned from the genetic dissection of stomatal, trichome and pavement cell formation, emerging methods in quantitative measurements that monitor cellular or tissue dynamics will allow us to further investigate cell state transitions and fate determination in leaf epidermal development. In this review, we introduce the formation of epidermal cell types in Arabidopsis and provide examples of quantitative tools to describe phenotypes in leaf research. We further focus on cellular factors involved in triggering cell fates and their quantitative measurements in mechanistic studies and biological patterning. A comprehensive understanding of how a functional leaf epidermis develops will advance the breeding of crops with improved stress tolerance.

Type
Review
Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (https://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution, and reproduction in any medium, provided the original work is properly cited.
Copyright
© The Author(s), 2022. Published by Cambridge University Press in association with The John Innes Centre

1. The epidermis as a load-bearing layer for organ morphogenesis

The ‘epidermal-growth-control’ or ‘tensile skin’ theory was proposed over a century ago based on the experimental result that the removal of the outer tissue (peripheral cell layers) resulted in a faster elongation of the inner stem tissue than with intact stems (Kutschera & Nikas, Reference Kutschera and Nikas2007). This observation suggested that the epidermis restricts organ growth. The molecular mechanism was then validated using epidermally expressed Brassinosteroids (BRs) signalling to promote cell expansion and rescue the dwarfism of br mutants (Savaldi-Goldstein et al., Reference Savaldi-Goldstein, Peto and Chory2007). The load-bearing epidermis is also required for organ integrity. A lack of coordination among the layers of the epidermis leads to cracks in tissues, but this phenotype can be fixed by reinforcing epidermal cell wall stiffness (Asaoka et al., Reference Asaoka, Ooe, Gunji, Milani, Runel, Horiguchi, Hamant, Sawa, Tsukaya and Ferjani2021; Verger et al., Reference Verger, Long, Boudaoud and Hamant2018). Recent studies and reviews have elucidated how mechanical forces shape plant organs and determined how tensile stress influences cell fate determination (Bidhendi et al., Reference Bidhendi, Altartouri, Gosselin and Geitmann2019; Malivert et al., Reference Malivert, Hamant and Ingram2018; Sampathkumar et al., Reference Sampathkumar, Krupinski, Wightman, Milani, Berquand, Boudaoud, Hamant, Jönsson and Meyerowitz2014; Trinh et al., Reference Trinh, Alonso-Serra, Asaoka, Colin, Cortes, Malivert, Takatani, Zhao, Traas, Trehin and Hamant2021; Yang et al., Reference Yang, Tran, Tsai and Ho2022). Here, we focus on the molecular mechanisms underlying epidermal fate determination and patterning using quantitative measurements at the tissue or cellular level.

2. Cell types of the leaf epidermis

The leaf epidermis in Arabidopsis comprises three cell types: trichomes, pavement cells, and stomata. Trichomes are hair-like structures on the leaf surface that offer a defensive barrier against herbivores and insects (Handley et al., Reference Handley, Ekbom and Agren2005). So-called pavement cells ‘pave’ the leaf surface, forming another physical barrier that prevents attacks by pathogens such as bacteria and fungi. Additionally, pavement cells are covered by a cuticle on their external side (facing the air) to reduce water loss through evaporation (Lu et al., Reference Lu, Zhao, Des Marais, Parsons, Wen, Xu, Bangarusamy, Wang, Rowland, Juenger, Bressan and Jenks2012). Arabidopsis stomata are valve-like pores on the leaf surface that are formed by a pair of kidney-shaped guard cells. They permit leaves to take up carbon dioxide from the atmosphere while allowing water evaporation, which drives water uptake from the roots. These three cell types coordinate their development and placement to form proper compartments to keep carbon dioxide for mesophyll cells to generate sucrose-based energy. Therefore, the leaf epidermis provides a barrier that protects mesophyll cells and is important for balancing water evaporation and carbon dioxide acquisition.

The precursor cells that form the leaf epidermis are derived from the outermost layer of the shoot apical meristem (SAM). The transcription factor WUSCHEL (WUS), whose encoding gene is expressed in the organising centre, interacts with CLAVATA1 (CLV1), CLV2 and CLV3 at the SAM (Clark et al., Reference Clark, Running and Meyerowitz1993, Reference Clark, Running and Meyerowitz1995; Fletcher et al., Reference Fletcher, Brand, Running, Simon and Meyerowitz1999; Kayes & Clark, Reference Kayes and Clark1998; Mayer et al., Reference Mayer, Schoof, Haecker, Lenhard, Jurgens and Laux1998). WUS and CLV establish a feedback loop that controls the size of the SAM and maintains the organising centre (Schoof et al., Reference Schoof, Lenhard, Haecker, Mayer, Jurgens and Laux2000). The central zone further differentiates into the L1 and L2 layers, with epidermal cells differentiating from L1, and mesophyll cells and fundamental stem tissues differentiating from L2. The homeobox-containing transcription factors ARABIDOPSIS THALIANA MERISTEM LAYER1 (ATML1) and PROTODERMAL FACTOR2 (PDF2) regulate the establishment of L1 (Abe et al., Reference Abe, Katsumata, Komeda and Takahashi2003). In Arabidopsis (Arabidopsis thaliana) leaves, the L1 layer forms the protoderm, which differentiates into trichomes, stomata, or puzzle piece–like pavement cells on the adaxial side of leaves or into stomata or pavement cells on the abaxial side (Figure 1a).

Fig. 1. Key factors involved in fate determination and leaf epidermal patterning during development. (A) Three trajectories describe the three distinct cell types of the leaf epidermis. The development and size of the shoot apical meristem (SAM) is controlled by the CLAVATA3 (CLV3)-WUSCHEL (WUS)-mediated negative feedback loop. The transcription factor (TF) genes ARABIDOPSIS THALIANA MERISTEM LAYER1 (ATML1) and PROTODERMAL FACTOR2 (PDF2) are expressed in the outermost layer (L1, blue) in the SAM to establish epidermal cell identity. Cells in the L1 layer called protoderms give rise to trichome-initiating cells (yellow), meristemoid mother cells (light blue), and pavement cells (grey). During trichome development, the major TF, GLABRA2 (GL2), drives cells to become polyploid trichome cells; the differentiation state is maintained by endoreduplication. To form a stomate, the master TF, SPEECHLESS (SPCH), initiates asymmetric cell division in a meristemoid mother cell to generate a small meristemoid (green) and a stomatal lineage ground cell (SLGC, white). MUTE then replaces SPCH and commits the cell to becoming a guard mother cell. Subsequently, FAMA in the guard mother cell drives symmetric cell division, resulting in a pair of guard cells. An SLGC can either undergo differentiation to become a pavement cell or divide asymmetrically again to produce another stomate (labelled by a dashed line). To date, no cell-type-specific driving factors have been associated with pavement cell formation. However, pavement cell maturation is often coupled with endoreduplication. (B) The cell–cell communication between trichome and non-trichrome cells relies on TRIPTYCHON (TRY). Before trichome initiation, GL1, GL3, and TRANSPARENT TESTA GLABRA1 (TTG1) form a stable MBW complex to activate GL2 transcription. GL2 accumulation promotes trichome cell fate. Besides GL2, the MBW complex also activates TRY expression in trichome cells. TRY tends to move to the neighbouring non-trichome cell to replace GL1 and disrupt the formation of the MBW complex, thus repressing GL2 and inhibiting the trichome cell fate. (C) Stomatal patterning follows the one-cell-spacing rule, meaning that two stomata never directly contact each other, and this signalling is mediated through peptide-mediated inhibitory signals and polarity establishment during stomatal development. SPCH drives the accumulation of a signalling peptide, EPIDERMAL PATTERNING FACTOR2 (EPF2), in meristemoids. The secreted peptides then bind to members of the receptor-like kinase ERECTA family and the receptor-like protein TMM on the surface of neighbouring cells. The binding triggers a MAPK cascade that phosphorylates and inhibits SPCH activity, thus preventing stomatal fate in these neighbouring cells. The interplay of chemical transduction and the polarity complex consisting of BASL, BREVIS RADIX-LIKE2 (BRXL2), and POLAR is required for asymmetric cell division and serves as a scaffold for recruiting and exerting inhibitory signalling in non-stomatal lineage cells. (D) Pavement cell formation is controlled biochemically by auxin. The high auxin concentration at the lobe initiation site induces the asymmetric accumulation of RHO-RELATED PROTEIN FROM PLANTS (ROP)-ROP-INTERACTIVE CRIB MOTIF-CONTAINING PROTEIN (RIC) in the two pavement cells. For the lobing cell (left), the recruitment of ROP2 and RIC4 helps the formation of actin filaments (F-actin) and further results in the protrusion of the cell. For the indented cell (right), ROP6 and RIC1 stabilise microtubule organisation under parallel direction and further pull the cell, forming an indentation.

2.1. Trichome development

Epidermal development is spatially and temporally regulated by cell fate factors, cell polarity and inhibitory signalling. For example, the development of initial trichome cells is controlled by GLABRA2 (GL2), a class IV homeodomain-containing basic leucine zipper (HD-bZIP) transcription factor (Rerie et al., Reference Rerie, Feldmann and Marks1994). GL2 promotes trichome maturation through cell expansion, branching, and cell wall establishment (Szymanski et al., Reference Szymanski, Jilk, Pollock and Marks1998). GL2 expression is activated by a complex, termed the MBW complex, which consists of the R2R3 MYB protein GL1, the basic helix-loop-helix (bHLH) transcription factor GL3, and the WD40-repeat protein TRANSPARENT TESTA GLABRA1 (TTG1) (Payne et al., Reference Payne, Zhang and Lloyd2000). The MBW complex activates GL2 transcription to induce trichome cell fate and promotes the translocation of the R3 MYB protein TRIPTYCHON (TRY) to neighbouring non-hair cells, where it replaces GL1 in the MBW complex (Schnittger et al., Reference Schnittger, Folkers, Schwab, Jurgens and Hulskamp1999; Zhao et al., Reference Zhao, Morohashi, Hatlestad, Grotewold and Lloyd2008). The MBW complex containing TRY represses GL2 expression and inhibits trichome initiation in non-hair cells (Schellmann et al., Reference Schellmann, Schnittger, Kirik, Wada, Okada, Beermann, Thumfahrt, Jurgens and Hulskamp2002; Schnittger et al., Reference Schnittger, Folkers, Schwab, Jurgens and Hulskamp1999; Figure 1b). In addition to this activator–inhibitor model, trichome patterning also requires an activator–depletion mechanism that traps TTG1 in trichome initial cells to enhance trichome production (Balkunde et al., Reference Balkunde, Deneer, Bechtel, Zhang, Herberth, Pesch, Jaegle, Fleck and Hulskamp2020; Digiuni et al., Reference Digiuni, Schellmann, Geier, Greese, Pesch, Wester, Dartan, Mach, Srinivas, Timmer, Fleck and Hulskamp2008; Pesch & Hulskamp, Reference Pesch and Hulskamp2009), which we discuss in more detail in Section 4.2.

2.2. Stomatal development

Stomatal development is driven by a transcription factor cascade starting with the related bHLH proteins SPEECHLESS (SPCH), MUTE, and FAMA (MacAlister et al., Reference MacAlister, Ohashi-Ito and Bergmann2007; Ohashi-Ito & Bergmann, Reference Ohashi-Ito and Bergmann2006; Pillitteri et al., Reference Pillitteri, Sloan, Bogenschutz and Torii2007). SPCH promotes asymmetric cell division in the protoderm, resulting in a small cell (meristemoid) and a large cell (stomatal lineage ground cell, SLGC) (MacAlister et al., Reference MacAlister, Ohashi-Ito and Bergmann2007; Pillitteri et al., Reference Pillitteri, Sloan, Bogenschutz and Torii2007). MUTE commits the meristemoid to the stomatal fate and activates the expression of genes involved in symmetric division and cell cycle regulation (Han et al., Reference Han, Qi, Sugihara, Dang, Endo, Miller, Kim, Miura and Torii2018; Reference Han, Herrmann, Yang, Iwasaki, Sakamoto, Desvoyes, Kimura, Gutierrez, Kim and Torii2022; Pillitteri et al., Reference Pillitteri, Sloan, Bogenschutz and Torii2007). FAMA then drives symmetric cell division to generate a pair of guard cells (Ohashi-Ito & Bergmann, Reference Ohashi-Ito and Bergmann2006). bHLH transcription factors typically associate as homodimers or heterodimers. SCREAM (SCRM) and SCRM2 function together with SPCH, MUTE and FAMA along this cell lineage to drive stomatal production (Kanaoka et al., Reference Kanaoka, Pillitteri, Fujii, Yoshida, Bogenschutz, Takabayashi, Zhu and Torii2008).

Stomatal distribution follows the one-cell-spacing rule; two stomata never directly touch each other and are thus separated by at least one cell. Cell-to-cell communication initiates from the meristemoid, which secretes the peptides EPIDERMAL PATTERNING FACTOR1 (EPF1) and EPF2. These peptides then bind to receptor protein kinases from the ERECTA family (ERf) and to the coreceptor TOO MANY MOUTHS (TMM). This receptor-coreceptor complex then activates a MITOGEN-ACTIVATED PROTEIN KINASE (MAPK) cascade that inhibits SPCH activity in SLGCs (Bergmann et al., Reference Bergmann, Lukowitz and Somerville2004; Hara et al., Reference Hara, Kajita, Torii, Bergmann and Kakimoto2007; Reference Hara, Yokoo, Kajita, Onishi, Yahata, Peterson, Torii and Kakimoto2009; Ho et al., Reference Ho, Paciorek, Abrash and Bergmann2016; Hunt & Gray, Reference Hunt and Gray2009; Lampard et al., Reference Lampard, Macalister and Bergmann2008; Lee et al., Reference Lee, Kuroha, Hnilova, Khatayevich, Kanaoka, McAbee, Sarikaya, Tamerler and Torii2012; Shpak et al., Reference Shpak, McAbee, Pillitteri and Torii2005). Polar proteins located in SLGCs, including BREAKING OF ASYMMETRY IN THE STOMATAL LINEAGE (BASL), members of the BREVIS RADIX family (BRXf), and POLAR (Dong et al., Reference Dong, MacAlister and Bergmann2009; Houbaert et al., Reference Houbaert, Zhang, Tiwari, Wang, de Marcos Serrano, Savatin, Urs, Zhiponova, Gudesblat, Vanhoutte, Eeckhout, Boeren, Karimi, Betti, Jacobs, Fenoll, Mena, de Vries, De Jaeger and Russinova2018; Pillitteri et al., Reference Pillitteri, Peterson, Horst and Torii2011; Rowe et al., Reference Rowe, Dong, Weimer and Bergmann2019), form a complex on the opposite side of the meristemoid and serve as a scaffold for recruiting the inhibitory signalling components MAPK3 and MAPK6 to phosphorylate and inhibit SPCH, thus preventing SLGCs from adopting a stomatal fate (Lampard et al., Reference Lampard, Macalister and Bergmann2008; Zhang et al., Reference Zhang, Wang, Shao, Zhu and Dong2015; Figure 1c). The resulting SLGCs can either become pavement cells or reinitiate several rounds of asymmetric divisions to produce a range of patterns on the epidermis (Gong, Alassimone, et al., Reference Gong, Alassimone, Varnau, Sharma, Cheung and Bergmann2021a; Ho et al., Reference Ho, Bringmann, Oshima, Mitsuda and Bergmann2021).

2.3. Pavement cell formation

Cells other than trichomes or stomatal initial cells differentiate into pavement cells. No cell-type-specific transcription factor has yet been described to be associated with pavement cell formation. Arabidopsis pavement cells take on their intriguing puzzle shape via the action of auxin gradients, cytoskeletal function, epidermal tension from cell proliferation and expansion, and the force from tissue growth (Grones et al., Reference Grones, Majda, Doyle, Van Damme and Robert2020; Sapala et al., Reference Sapala, Runions, Routier-Kierzkowska, Das Gupta, Hong, Hofhuis, Verger, Mosca, Li, Hay, Hamant, Roeder, Tsiantis, Prusinkiewicz and Smith2018; Xu et al., Reference Xu, Wen, Nagawa, Fu, Chen, Wu, Perrot-Rechenmann, Friml, Jones and Yang2010; Reference Xu, Dai, Chen, Nagawa, Cao, Li, Zhou, Chen, De Rycke, Rakusova, Wang, Jones, Friml, Patterson, Bleecker and Yang2014). Pavement cell interdigitation is abolished in mutants lacking auxin biosynthesis function or the auxin efflux transporter PIN-FORMED1 (PIN1) (Xu et al., Reference Xu, Wen, Nagawa, Fu, Chen, Wu, Perrot-Rechenmann, Friml, Jones and Yang2010). Auxin actives two Rho GTPases that promote the formation of the complementary lobes and indentations. The GTPase RHO OF PLANTS2 (ROP2) and ROP-INTERACTIVE CRIB MOTIF-CONTAINING PROTEIN4 (RIC4) activate F-actin formation for the protrusion of lobes, while ROP6 and RIC1 promote microtubule organisation for indentations (Fu et al., Reference Fu, Xu, Zhu, Wen and Yang2009). The bridge between auxin and the action of Rho GTPase signalling is AUXIN BINDING PROTEIN1 (ABP1), which interacts with the plasma membrane–localised receptor-like transmembrane kinases (TMKs), leading to the activation of Rho GTPases and the formation of the puzzle shapes characteristic of pavement cells on the surface of Arabidopsis leaves (Xu et al., Reference Xu, Dai, Chen, Nagawa, Cao, Li, Zhou, Chen, De Rycke, Rakusova, Wang, Jones, Friml, Patterson, Bleecker and Yang2014; Figure 1d).

The cell cycle provides an additional layer of control in epidermal cell fate determination and maintenance. For example, the formation of pavement cells and trichomes is usually associated with increased ploidy; however, stomatal cells remain diploid (Larson-Rabin et al., Reference Larson-Rabin, Li, Masson and Day2009; Melaragno et al., Reference Melaragno, Mehrotra and Coleman1993; Xu et al., Reference Xu, Dai, Chen, Nagawa, Cao, Li, Zhou, Chen, De Rycke, Rakusova, Wang, Jones, Friml, Patterson, Bleecker and Yang2014; Zuch et al., Reference Zuch, Doyle, Majda, Smith, Robert and Torii2022). The mitotic cell cycle comprises G1, S, G2, and M phases and results in two diploid (2n) daughter cells; endoreplication, a specialised type of cell cycle, increases ploidy (4n, 8n, 16n, or more) by undergoing DNA replication by skipping cell division. Endoreplication is crucial for trichome fate maintenance (Bramsiepe et al., Reference Bramsiepe, Wester, Weinl, Roodbarkelari, Kasili, Larkin, Hülskamp and Schnittger2010). When CYCLIN-DEPENDENT KINASE A;1 (CDKA;1) is mutated or when the CDK inhibitor KIP-RELATED PROTEIN1 (KRP1, also named INHIBITOR/INTERACTOR WITH CYCLIN-DEPENDENT KINASE1 [ICK1]) is ectopically and stably expressed, trichomes only undergo mitotic division; these plants have fewer trichomes and these trichomes have fewer branches (Bramsiepe et al., Reference Bramsiepe, Wester, Weinl, Roodbarkelari, Kasili, Larkin, Hülskamp and Schnittger2010).

In the following sections, we summarise quantitative methods for characterising leaves, trichomes, stomata, and pavement cells as well as protein polarity and cell cycle progression (Table 1). By obtaining quantitative data, we can then trace the transitions between cell states and start to understand cell decisions over the course of development.

Table 1 Quantitative tools to measure leaf epidermis features

3. Quantitative methods to study leaves

3.1. Leaf shape

Arabidopsis forms elliptical true leaves with a serrated edge. Classical parameters such as leaf area, length (height), width, and circularity are used to describe leaf shapes. The ratio between the length and width determines whether the leaf is more circular or elliptical. Leaf circularity reflects the degree of serration of the leaf margin (Figure 2a). The program LAMINA (Leaf shApe deterMINAtion) was developed in 2008 to extract such leaf measurements from scanned leaf images and performs well on both single and compound leaves (Bylesjo et al., Reference Bylesjo, Segura, Soolanayakanahally, Rae, Trygg, Gustafsson, Jansson and Street2008). LAMINA can be employed to determine the number of leaf serrations and boundary coordinates, which describe the degree of asymmetry in leaf shape. However, LAMINA cannot detect petioles or describe highly complex leaves. In Arabidopsis, there is no clear boundary between the leaf blade and petiole, which may hinder the quantification of overall leaf area (which would include the petiole here). Using the program MorphoLeaf, the petiole can be removed manually to increase the accuracy of leaf shape quantification (Biot et al., Reference Biot, Cortizo, Burguet, Kiss, Oughou, Maugarny-Cales, Goncalves, Adroher, Andrey, Boudaoud and Laufs2016). Furthermore, landmark-guided reparameterization in MorphoLeaf enables the determination of the average leaf shape based on several biological samples. This feature is useful when tracing leaf developmental trajectories and obtaining morphometrics. Many classical parameters can be collected and analysed in a principal component analysis (PCA) to investigate the main differences between plant species, varieties, or accessions. The GUI (graphical user interface)–based package LeafI (Leaf Interrogator) in the Python environment can also be used to analyse leaf images and generate datasets in which classical leaf shape parameters are assembled (Zhang et al., Reference Zhang, Runions, Mentink, Kierzkowski, Karady, Hashemi, Huijser, Strauss, Gan, Ljung and Tsiantis2020). Moreover, LeafI provides statistical analysis and visualisation tools to facilitate and accelerate analysis. The PCA function of LeafI can clearly detect differences in leaf shape between mutants. For example, an analysis of single and higher-order mutants of the WUSCHEL-RELATED HOMEOBOX (WOX) family, the latter of which have spindle-like leaves, indicated that WOX proteins are required for lateral leaf expansion (Zhang et al., Reference Zhang, Runions, Mentink, Kierzkowski, Karady, Hashemi, Huijser, Strauss, Gan, Ljung and Tsiantis2020).

Fig. 2. Quantitative methods to describe leaf morphology and the different types of epidermal cells. (A) Leaf shape can be described by its length, width, and the length/width ratio. Circularity calculated by (4 $\pi$ ×leaf area)/(square perimeter) indicates that the leaf shape is approximately round (circularity = 1) or contains serrations (circularity closer to 0). If serrations are visible on a leaf, the indent length and width can be used to describe the extent of serration. (B) Trichome phenotypes can be measured by the number of trichomes on a leaf and trichome morphology. Trichome density can be scored over an entire leaf or a given area. Trichome index is the number of trichomes divided by the number of total epidermal cells including trichome, stomatal, and pavement cells over a given area. The trichome stalk, the branching number, and the branching points can be used to represent trichome shape. The trichome branching index represents the average number of branches in a trichome population. (C) Stomatal phenotypes can be described by stomatal number, pattern, and dynamics. Stomatal density represents the number of stomata over a given area. The stomatal index is defined as the number of stomata divided by the total number of epidermal cells. Stomatal groups are the number of stomatal islands in a given area. Adjacent stomata are defined as one group. A cluster event represents the number of islands with adjacent stomata. Cluster frequency represents the error rate of forming stomatal clusters. The movements of stomata can be described by stomatal length and width. Pore length and width excluding guard cells may also be used. During stomatal opening, the stomatal and pore lengths decrease, while the pore width increases. (D) Pavement cell phenotypes can be described according to their shape including the parameters of area, perimeter, length and width. The aspect ratio calculates the ratio between cell length and width. The jigsaw-puzzle shape can be described by the number of lobes and indentations, which can be expressed as circularity, solidity, and completeness. Circularity is calculated as (4 $\pi$ ×cell area)/(square perimeter). Solidity is the ratio between cell area and convex hull area. Completeness is the ratio between visible and total possible links. A visible link represents the link between two nodes without crossing over the cell outline. An invisible link is defined as a link between two nodes that crosses over the cell outline. All three parameters have maxima equal to 1. They decrease when the cell takes on the shape of a jigsaw-puzzle piece.

Besides the classical leaf shape parameters, the program LIMANI (Leaf IMage ANalysis Interface) provides information about the vascular patterns of leaves (Dhondt et al., Reference Dhondt, Van Haerenborgh, Van Cauwenbergh, Merks, Philips, Beemster and Inze2012). Using ethanol-cleared leaves and darkfield images to increase image contrast is critical for analyses via LIMANI, which can score vascular density, the number of branching points, and the number of lamina and areola. Combined with classical parameters, measuring these additional parameters may improve our understanding of the relationship between vein and shape developments.

Because Arabidopsis leaves are flat, most programs focus on two-dimensional (2D) leaf structures. Remmler and Rolland-Lagan (Reference Remmler and Rolland-Lagan2012) computationally quantified the three-dimensional (3D) structure (curvature) of the leaf adaxial surface using brightfield and fluorescence z-stack images (Remmler & Rolland-Lagan, Reference Remmler and Rolland-Lagan2012). In a study of the development of the first true leaf in Arabidopsis, the 3D structure of the leaf changed due to spatial heterogeneity in growth, even when the classical leaf shape parameters did not appear to change significantly (Rolland-Lagan et al., Reference Rolland-Lagan, Remmler and Girard-Bock2014). This model may elucidate the relationship between growth and shape and the effects of mechanical properties on the leaf surface.

3.2. Trichomes

In Arabidopsis, trichomes are present on the adaxial side of true leaves but not on cotyledons. Mutations in genes associated with trichome development influence the number or presence of trichomes (Payne et al., Reference Payne, Zhang and Lloyd2000; Rerie et al., Reference Rerie, Feldmann and Marks1994). Trichomes with fewer branches are observed in plants with mutations in genes associated with cytoskeleton organisation or endoreplication (Roodbarkelari et al., Reference Roodbarkelari, Bramsiepe, Weinl, Marquardt, Novák, Jakoby, Lechner, Genschik and Schnittger2010; Tian et al., Reference Tian, Han, Feng, Wang, Liu, Ma, Yu and Kong2015). Their individual shape and their spatial organisation can be described using different sets of parameters. The cell proportion is usually calculated as trichome density (number per leaf or per given area). However, given that bigger cells can result in lower cell counts, the trichome index can be used to eliminate the size effect, which is the number of trichomes divided by the total number of epidermal cells (trichome + stomatal + pavement cells) (Figure 2b).

Trichome morphology can be described by the properties of trichome stalks and branches. Stalk length and diameter can be extracted from trichome images taken with a scanning electron microscope (Szymanski et al., Reference Szymanski, Marks and Wick1999). Zhang and Oppenheimer (Reference Zhang and Oppenheimer2004) developed a simple method to isolate trichomes from leaves and observe them under light microscopy. Using the definition of stalk length as the distance from the basal cells to the first branching point and branch length as the distance between branching points, Zhang et al. (Reference Zhang, Grey, Krishnakumar and Oppenheimer2005) reported that a mutation in IRREGULAR TRICHOME BRANCH (ITB) resulted in a cell expansion defect with no effect on the branching pattern. Branching can be described as the number of branches and branching points for a mature trichome (Figure 2b). Typically, Arabidopsis trichomes have three branches with two branching points (Abe et al., Reference Abe, Thitamadee and Hashimoto2004). If branching is highly variable between individual cells, the branching index can be used as a metric, which is calculated as the total number of branches (k) multiplied by the number of trichomes with k branches and divided by the total number of trichomes (Figure 2b; Vadde et al., Reference Vadde, Challa and Nath2018). The branching index thus represents the average number of branch points in a trichome.

Trichome patterning is a critical character to describe the epidermis. Clusters of trichomes occur in mutants defective in endoreplication, such as the siamese (sim) mutants (Walker et al., Reference Walker, Oppenheimer, Concienne and Larkin2000), or mutants in repressors of trichome development, such as try mutants (Schnittger et al., Reference Schnittger, Folkers, Schwab, Jurgens and Hulskamp1999). Except for strongly abnormal phenotypes, such as contiguous trichome clustering, uneven distributions of trichomes along the leaf surface can be described. The point-pattern approximation that we refer uses the nearest neighbour distance (NND), where each individual trichome/stomate is considered as a point (Clark & Evans, Reference Clark and Evans1954). Okamoto et al. (Reference Okamoto, Negishi, Toyama, Ushijima and Morohashi2020) used the point–pattern approximation and a GL3pro:GL3-GFP reporter to monitor gene expression under control and heat treatments. They observed that the trichome patterning gene GL3 is expressed heterogeneously. This finding suggested that the noise resulting from either the abundance of cellular components or environmental conditions may lead to variable patterns in a biological system (Okamoto et al., Reference Okamoto, Negishi, Toyama, Ushijima and Morohashi2020). Therefore, to predict the regulatory pathways underlying the formation of a given pattern, this variability needs to be considered. Greese et al. (Reference Greese, Hulskamp and Fleck2014) reviewed several methods using the point pattern approximation. By comparing the experimental data and simulation of activator mobility in trichome initiation, they found that with the increasing activator mobility, the local noise decreases and the trichome pattern becomes more regular, illustrating less variability. It suggests that even a highly regulated biological process can be substantially affected by variability, which may explain the known high flexibility of plant development.

3.3. Stomata

Stomatal distribution is an example of biological patterning. To describe the stomatal patterns (clustered, even, or random) in different species, the point–pattern approximation similar to the described analysis in trichomes is often used. However, in the case of stomata on the surface of the leaf epidermis (shown in Figure 2), the size of one stomate limits the placing of neighbouring cells. The disk–NND (disk–null model) method considers the influence of stomatal size (Naulin et al., Reference Naulin, Valenzuela and Estay2017). Results from the disk–null model are indeed more accurate than a simple NND approach in defining stomatal clusters in Arabidopsis, which has a high stomatal density (Naulin et al., Reference Naulin, Valenzuela and Estay2017).

Epidermal patterning can be visualised by staining with propidium iodide or using plasma membrane markers to delineate the outline of epidermal cells. Yang et al. (Reference Yang, Tran, Tsai and Ho2022) applied five measurements to systematically describe stomata: stomatal density, stomatal index, stomatal group, cluster event, and cluster frequency. Stomatal density is the number of stomata in a given area. To remove the effect of the expansion of pavement cells from both stomatal and non-stomatal lineages, the stomatal index represents the number of stomata as a proportion of the total number of epidermal cells. The stomatal density and index are influenced by the number of initial stomatal cells and adjacent stomatal clusters, which are derived from the same origin of asymmetrically divided sister cells (a single stomatal group). Therefore, the number of stomatal groups reflects the initial number of stomatal formation events. A stomatal cluster event is the number of stomatal clusters with more than two adjacent stomata. The cluster frequency is the ratio between the number of stomatal cluster events and stomatal groups and indicates the error rate of cluster formation (Figure 2c). To describe the stomatal arrangement, stomatal evenness using the method of minimum spanning tree, stomatal divergence using the method of distance to the gravity and stomatal aggregation using NND were proposed (Liu et al., Reference Liu, Li, Xu, Li, Wang, Yan and He2021). Based on the simulation results, the stomatal divergence is influenced by the stomatal number while stomatal evenness and stomatal aggregation are more consistent in the stomatal number ranging from 15 to 50 (Liu et al., Reference Liu, Li, Xu, Li, Wang, Yan and He2021). Since the placement of stomata can be more regular in monocot than in dicot plants, plant species should be considered when making a comparison. The stomatal production and patterning are influenced by the environment, therefore, using the aforementioned methods to study the patterns of stomatal distribution may reflect their development, adaptation, and even evolution.

Stomatal conductance is a measure of the degree of stomatal opening and can be monitored as a sum of stomatal responses in a leaf using a photosynthesis system (Li-Cor system). Therefore, to directly probe changes in stomatal apertures, opening and closing events are measured at the cellular level under a microscope. Because Arabidopsis stomata are approximately elliptical, they can be described by the length and width or the area of their aperture (Figure 2c). Changes in stomatal size or stomatal aperture under various environmental conditions can be measured to investigate the response speed of stomata (Nagatoshi et al., Reference Nagatoshi, Mitsuda, Hayashi, Inoue, Okuma, Kubo, Murata, Seo, Saji, Kinoshita and Ohme-Takagi2016; Tsai et al., Reference Tsai, Kuan, Guo, Yang, Chung and Ho2022).

3.4. Pavement cells

Pavement cells make up the bulk of the leaf surface and interlock with each other like a jigsaw puzzle. This pattern is created and maintained by an auxin-mediated pathway and the mechanical stress between epidermal cells (Sapala et al., Reference Sapala, Runions, Routier-Kierzkowska, Das Gupta, Hong, Hofhuis, Verger, Mosca, Li, Hay, Hamant, Roeder, Tsiantis, Prusinkiewicz and Smith2018; Xu et al., Reference Xu, Wen, Nagawa, Fu, Chen, Wu, Perrot-Rechenmann, Friml, Jones and Yang2010). The interdigitation of the lobes and indentations provides balance between the growth direction of two neighbouring cells (Sapala et al., Reference Sapala, Runions, Routier-Kierzkowska, Das Gupta, Hong, Hofhuis, Verger, Mosca, Li, Hay, Hamant, Roeder, Tsiantis, Prusinkiewicz and Smith2018). Modulating cell wall stiffness also plays a role in shaping pavement cells through controlling pectin composition (Altartouri et al., Reference Altartouri, Bidhendi, Tani, Suzuki, Conrad, Chebli, Liu, Karunakaran, Scarcelli and Geitmann2019; Haas et al., Reference Haas, Wightman, Meyerowitz and Peaucelle2020). Therefore, the morphology of pavement cells may serve as a proxy for the mechanical properties of the leaf epidermis. Several parameters have been used to describe pavement cells, including the aspect ratio, the number of lobes and indentations, circularity, solidity, and convexity (Figure 2d). PaCeQuant, LobeFinder and LOCO-EFA all use a boundary-based approach to detect the lobes (Möller et al., Reference Möller, Poeschl, Plötner and Bürstenbinder2017; Sanchez-Corrales et al., Reference Sanchez-Corrales, Hartley, van Rooij, Maree and Grieneisen2018; Wu et al., Reference Wu, Belteton, Pack, Szymanski and Umulis2016). Among them, PaCeQuant, an ImageJ-based tool, provides 27 pavement cell-shape features (Möller et al., Reference Möller, Poeschl, Plötner and Bürstenbinder2017). PaCeQuant either automatically detects cell boundaries of pavement cells from a confocal image or uses an input file with segmented cells. In PaCeQuant, circularity is defined as 4 $\pi$ multiplied by the area of a pavement cell divided by the squared perimeter (Figure 2d). Convexity is defined as the perimeter of the convex hull divided by the perimeter of the cell. Solidity is defined as the area of the convex hull divided by the area of the cell (Möller et al., Reference Möller, Poeschl, Plötner and Bürstenbinder2017). These three parameters represent the lobing degree of a cell. They can be used together with pavement cell area, perimeter, and length/width ratio to generate a phylogeny map based on pavement cell shapes (Vofely et al., Reference Vofely, Gallagher, Pisano, Bartlett and Braybrook2019).

GraVis is a Python 3.0 tool that uses a visibility map (Figure 2d) in a network-based approach to describe pavement cells (Nowak et al., Reference Nowak, Eng, Matz, Waack, Persson, Sampathkumar and Nikoloski2021). The outline of a pavement cell is equally marked with several nodes (Figure 2d). A link is visible when it connects two nodes without crossing the cell outline, while invisible links cross the cell outline. A local maximum (more visible links) indicates indentation, and a local minimum (fewer links) indicates a lobe. A visibility matrix (the correlation between every node, including their link lengths) and completeness (the ratio between all possible links and the actual number of links) can be used to group similar shapes together and describe the lobing degree of a pavement cell (Nowak et al., Reference Nowak, Eng, Matz, Waack, Persson, Sampathkumar and Nikoloski2021).

3.5. Large-scale, time-lapse tracking

Quantitative cell imaging provides unique spatial and temporal information at the cellular level in a multicellular context; however, it requires a huge amount of analytic power. A trend of developing computational tools to efficiently measure and extract valuable information on biological phenotypes and dynamics is emerging. Some tools used for the quantification of leaf epidermal images are listed in this section. StomataCounter was developed to automatically count stomata (Fetter et al., Reference Fetter, Eberhardt, Barclay, Wing and Keller2019). The input files can be images from differential interference contrast microscopy and brightfield observations. This tool is useful for field-collected specimens in which no fluorescent dye can be deployed easily to mark the cell outline. Because the method requires high-quality images, those below a given quality cut-off need to be eliminated to obtain reliable results.

To measure and quantify the properties of every cell in a growing tissue, the accurate segmentation of individual cells from volumetric images is required. Therefore, leaves stained with propidium iodide or transgenic plants expressing a fluorescent plasma membrane marker are usually used to increase the contrast of images. The image segmentation tools Cellpose (Stringer et al., Reference Stringer, Wang, Michaelos and Pachitariu2021) and PlantSeg allow performing 3D cell segmentation and extract quantitative measures at the single cell level (Wolny et al., Reference Wolny, Cerrone, Vijayan, Tofanelli, Barro, Louveaux, Wenzl, Strauss, Wilson-Sanchez, Lymbouridou, Steigleder, Pape, Bailoni, Duran-Nebreda, Bassel, Lohmann, Tsiantis, Hamprecht, Schneitz and Kreshuk2020). Because a stomate is composed of two guard cells, the two guard cells are considered individual cells rather than a single stomate when working on cellular segmentation. To solve this problem, LeafNet applies a hierarchical strategy to first identify stomata and then segment pavement cells using stomata-masked images (Li et al., Reference Li, Li, Fan, Ma, Zhang, Kim, Wang, Russinova, Zhu and Zhou2022). Therefore, LeafNet can be used to obtain cell counts and sizes of individual stomata as well as pavement cells in a single analysis of a two-dimensional image.

MorphoGraphX (MGX) is a platform that analyzes morphogenesis from biological images (de Reuille et al., Reference de Reuille, Routier-Kierzkowska, Kierzkowski, Bassel, Schüpbach, Tauriello, Bajpai, Strauss, Weber, Kiss, Burian, Hofhuis, Sapala, Lipowczan, Heimlicher, Robinson, Bayer, Basler, Koumoutsakos and Smith2015; Strauss et al., Reference Strauss, Runions, Lane, Eschweiler, Bajpai, Trozzi, Routier-Kierzkowska, Yoshida, da Silveira, Vijayan, Tofanelli, Majda, Echevin, Le Gloanec, Bertrand-Rakusova, Adibi, Schneitz, Bassel, Kierzkowski and Smith2022). The recent MGX2.0 version implements the local coordinate system to a growing tissue or organ (Strauss et al., Reference Strauss, Runions, Lane, Eschweiler, Bajpai, Trozzi, Routier-Kierzkowska, Yoshida, da Silveira, Vijayan, Tofanelli, Majda, Echevin, Le Gloanec, Bertrand-Rakusova, Adibi, Schneitz, Bassel, Kierzkowski and Smith2022). By adding such spatial information, the measurements of cell size and shape as well as gene expression at single time points or cell proliferation and growth rates over time allow quantification in a living organism and comparison between cell types. This advanced implementation has facilitated the identification of growth differences between leaves and sepals. In sepals, growth is more distal in the early stages and then moves towards the base as the sepal develops (Strauss et al., Reference Strauss, Runions, Lane, Eschweiler, Bajpai, Trozzi, Routier-Kierzkowska, Yoshida, da Silveira, Vijayan, Tofanelli, Majda, Echevin, Le Gloanec, Bertrand-Rakusova, Adibi, Schneitz, Bassel, Kierzkowski and Smith2022). By contrast, the proliferation and expansion zones are relatively fixed in a proximal-distal fashion along the leaf length during leaf development (Fox et al., Reference Fox, Southam, Pantin, Kennaway, Robinson, Castorina, Sanchez-Corrales, Sablowski, Chan, Grieneisen, Maree, Bangham and Coen2018). Since cells with a common biological function tend to have similar geometric, positional, and expression attributes, the integration of positional information and shape morphology can substantially aid in assigning cell fate (Strauss et al., Reference Strauss, Runions, Lane, Eschweiler, Bajpai, Trozzi, Routier-Kierzkowska, Yoshida, da Silveira, Vijayan, Tofanelli, Majda, Echevin, Le Gloanec, Bertrand-Rakusova, Adibi, Schneitz, Bassel, Kierzkowski and Smith2022). For example, the coordinate system in a radially symmetric tissue makes it possible to distinguish between the epidermis, the cortex, and the stele in a root. The Arabidopsis gynoecium consists of the replum and lateral valves tissue, which has stomata (Strauss et al., Reference Strauss, Runions, Lane, Eschweiler, Bajpai, Trozzi, Routier-Kierzkowska, Yoshida, da Silveira, Vijayan, Tofanelli, Majda, Echevin, Le Gloanec, Bertrand-Rakusova, Adibi, Schneitz, Bassel, Kierzkowski and Smith2022). Therefore, the organ coordinates can first help identify a region of interest and then use cell geometry to distinguish stomata from other elongated cells (Strauss et al., Reference Strauss, Runions, Lane, Eschweiler, Bajpai, Trozzi, Routier-Kierzkowska, Yoshida, da Silveira, Vijayan, Tofanelli, Majda, Echevin, Le Gloanec, Bertrand-Rakusova, Adibi, Schneitz, Bassel, Kierzkowski and Smith2022). Moreover, advanced geometric analysis in time-lapse data such as lineage tracking, growth analysis, and cell division analysis in MGX2.0 will improve our understanding of spatiotemporal dynamics of cellular behaviours in the context of a developing organ.

4. Factors associated with cell fate determination and epidermal patterning

Cell geometry and dynamics such as polarity, cell cycle, cell size, cell division, and intercellular signalling such as cell-to-cell communication and auxin are known to play a role in cell fate determination and ultimately lead to the establishment of a biological pattern. Here, we introduce their functions in plant epidermal fate acquisition with a focus on quantitative measurements and the use of such quantitative data in understanding epidermal development.

4.1. Polarity

Spatiotemporal control is important for triggering different cell fates in asymmetrically dividing sister cells. During stomatal development, a polarly localised protein is required in SLGCs after asymmetric cell division for the MAPK-mediated repression of SPCH activity and the inhibition of stomatal formation (Dong et al., Reference Dong, MacAlister and Bergmann2009; Zhang et al., Reference Zhang, Wang, Shao, Zhu and Dong2015). Loss of function in polarly localised proteins such as BASL or its interacting proteins belonging to the BRX family results in stomatal clusters (Dong et al., Reference Dong, MacAlister and Bergmann2009; Rowe et al., Reference Rowe, Dong, Weimer and Bergmann2019). Cortical-localised BASL was shown to form a scaffold that recruits the MAPK KINASE KINASE (MAPKKK) YODA and MPK3/6 to activate signalling at the cortex (Zhang et al., Reference Zhang, Wang, Shao, Zhu and Dong2015). The activation of MAP kinase signalling at the polarised site, therefore, reinforces the feedback loop between BASL polarisation at the cortex and the inhibition of SPCH in the nucleus (Zhang et al., Reference Zhang, Wang, Shao, Zhu and Dong2015). BR signalling is also a regulator of stomatal production, although the underlying mechanism is more complex (Gudesblat et al., Reference Gudesblat, Schneider-Pizoń, Betti, Mayerhofer, Vanhoutte, van Dongen, Boeren, Zhiponova, de Vries, Jonak and Russinova2012; Kim et al., Reference Kim, Michniewicz, Bergmann and Wang2012). BR acts as a positive regulator by inhibiting the MAPK cascade, leading to the over-accumulation of SPCH and stomatal formation (Kim et al., Reference Kim, Michniewicz, Bergmann and Wang2012). However, BR can also be a negative regulator by directly phosphorylating and destabilising SPCH (Gudesblat et al., Reference Gudesblat, Schneider-Pizoń, Betti, Mayerhofer, Vanhoutte, van Dongen, Boeren, Zhiponova, de Vries, Jonak and Russinova2012). This dual role was solved by looking at the subcellular distribution of BRASSINOSTEROID INSENSITIVE2 (BIN2), a GLYCOGEN SYNTHASE KINASE3 (GSK3)/SHAGGY-like kinase, before and after asymmetric cell division (Houbaert et al., Reference Houbaert, Zhang, Tiwari, Wang, de Marcos Serrano, Savatin, Urs, Zhiponova, Gudesblat, Vanhoutte, Eeckhout, Boeren, Karimi, Betti, Jacobs, Fenoll, Mena, de Vries, De Jaeger and Russinova2018). BIN2 suppresses BR signalling by relocating from the cytosol to the nucleus to inhibit BR downstream transcription factors (He et al., Reference He, Gendron, Yang, Li and Wang2002; Kim et al., Reference Kim, Guan, Sun, Deng, Tang, Shang, Sun, Burlingame and Wang2009). One of the scaffold proteins, POLAR (Pillitteri et al., Reference Pillitteri, Peterson, Horst and Torii2011), spatially modulates the nucleo-cytoplasmic partitioning of BIN2 in the stomatal lineage. Before asymmetric division, BIN2 interacts with the polarity complex at the cortex. While this interaction is disrupted after asymmetric cell division, BIN2 relocates to the nucleus to destabilise SPCH in SLGCs, leading to asymmetric cell fates (Guo & Dong, Reference Guo and Dong2019; Houbaert et al., Reference Houbaert, Zhang, Tiwari, Wang, de Marcos Serrano, Savatin, Urs, Zhiponova, Gudesblat, Vanhoutte, Eeckhout, Boeren, Karimi, Betti, Jacobs, Fenoll, Mena, de Vries, De Jaeger and Russinova2018). Besides BIN2, recent work on the BRI1 SUPPRESSOR1-LIKE (BSL) family of protein phosphatases has also revealed that the spatial modulation of MAPK signalling at the subcellar level is key for asymmetric fate acquisition (Guo et al., Reference Guo, Park, Wang, Nickels and Dong2021; Reference Guo, Ding and Dong2022).

Plant cell polarity and tissue mechanics is an emerging field that needs to be taken into account for both biochemical and mechanical signalling in plant development (for reviews please see (Gorelova et al., Reference Gorelova, Sprakel and Weijers2021; Ramalho et al., Reference Ramalho, Jones, Mutte and Weijers2022). The polarity degree of the crescent length normalised to cell perimeter can be used to quantify the crescent size (Gong, Varnau, et al., Reference Gong, Varnau, Wallner, Acharya, Bergmann and Cheung2021b; Zhang et al., Reference Zhang, Wang, Shao, Zhu and Dong2015; Figure 3a). A smaller crescent size reflects a lower inhibitory effect on SPCH, leading to over-proliferation of stomata (Yang et al., Reference Yang, Tran, Tsai and Ho2022; Zhang et al., Reference Zhang, Wang, Shao, Zhu and Dong2015). Misoriented polarity can also disrupt stomatal patterning (Yang et al., Reference Yang, Tran, Tsai and Ho2022). Indeed, the degree of polarity of the polar protein BRX-like2 (BRXL2) in the leaf epidermis varies depending on its tissue location (Bringmann & Bergmann, Reference Bringmann and Bergmann2017). At the leaf base, BRXL2 tends to face towards the midrib in both the left and right halves of the leaf; therefore, the angle between the midrib and the direction of the BRXL2 crescent can be used to measure the tissue-wide orientation of polarity proteins (Bringmann & Bergmann, Reference Bringmann and Bergmann2017; Yang et al., Reference Yang, Tran, Tsai and Ho2022; Figure 3a). The migration of nuclei that is polarity-driven and mediated by microtubules and actin is also important for setting up asymmetric cell division (Muroyama et al., Reference Muroyama, Gong and Bergmann2020).

Fig. 3. Quantitative tools for measuring polarity and the cell cycle. (A) Polarity measurements. (i) The polarity degree is calculated by the crescent length (green) relative to the cell perimeter (green+pink). M: meristemoid. SLGC, stomatal lineage ground cell. (ii) Workflow for Polarity Measurement (POME), a Fiji-based semi-automated pipeline for polarity quantification: First, a line of 0° to 180° angle is defined by the centroid to the centre of polar protein mass. Second, the cell outline is reconstructed and visualised by quantification of the fluorescence intensity. Third, standard deviation (SD, $\sigma$ ), amplitude ( $\alpha$ ), and baseline intensity ( $\beta$ ) derived from the fluorescence intensity through Gaussian fitting quantify the degree of polarisation in the plasma membrane, with higher SD values representing higher polarity levels. (iii) Tissue-wide polarity orientation can be indicated by the angle (α) between the leaf midrib and the connection between the cell centroid (orange dot) and the midpoint of the polarity crescent. (B) Cell cycle measurements. (i) Cytrap (Cell cycle tracking in plant cells) line. The dual-colour cell cycle reporter line uses HTR2pro:CDT1a-RFP and CYCB1pro:CYCB1-GFP to indicate S/G2 and G2/M, respectively. (ii) PlaCCI (Plant Cell Cycle Indicator) line. The three-colour cell cycle reporter line adopted CDT1apro:CDT1a-CFP, CYCB1:1pro:CYCB1;1-YFP, and HTR13pro:HTR13-mCherry to indicate G1, G2/M, and the entire cell cycle, respectively.

Post-embryonic patterning is a dynamic process that depends on cell rearrangements, polarity, asymmetric division, and growth. The information collected from time-lapse imaging to trace the expression of SPCH and the dynamic location of the polarity protein BASL was assembled into a model that revealed a postmitotic polarity-switch mechanism that governs plant stem cells to generate their neighbours while spacing themselves apart (Robinson et al., Reference Robinson, de Reuille, Chan, Bergmann, Prusinkiewicz and Coen2011).

4.2. Cell-to-cell communication

Trichome distribution is mediated by the intercellular mobility of several patterning proteins. Many inhibitors, such as TRY, CAPRICE (CPC), and ENHANCER OF TRY AND CPC (ETC), can move between cells (Digiuni et al., Reference Digiuni, Schellmann, Geier, Greese, Pesch, Wester, Dartan, Mach, Srinivas, Timmer, Fleck and Hulskamp2008; Kurata et al., Reference Kurata, Ishida, Kawabata-Awai, Noguchi, Hattori, Sano, Nagasaka, Tominaga, Koshino-Kimura, Kato, Sato, Tabata, Okada and Wada2005; Wester et al., Reference Wester, Digiuni, Geier, Timmer, Fleck and Hulskamp2009; Zhao et al., Reference Zhao, Morohashi, Hatlestad, Grotewold and Lloyd2008). Among the activators (TTG1, GL1, and GL3), only TTG1 can move from cell to cell (Bouyer et al., Reference Bouyer, Geier, Kragler, Schnittger, Pesch, Wester, Balkunde, Timmer, Fleck and Hulskamp2008). TTG1 was shown to be depleted around trichomes in wild-type plants but not in gl3 mutants, suggesting that GL3 traps TTG1 in trichomes, where its encoding gene is strongly expressed (Bouyer et al., Reference Bouyer, Geier, Kragler, Schnittger, Pesch, Wester, Balkunde, Timmer, Fleck and Hulskamp2008). Two models have been proposed to explain trichome patterning: the activator–inhibitor model and the activator–depletion model (Pesch & Hulskamp, Reference Pesch and Hulskamp2009). The activator–inhibitor model posits that the activator complex promotes the production of inhibitors that move to the neighbouring cells, where they repress trichome formation, as shown in Figure 1b. The activator–depletion model assumes the trapping of mobile TTG1 by GL3 in incipient trichomes, thus enhancing trichome production (Digiuni et al., Reference Digiuni, Schellmann, Geier, Greese, Pesch, Wester, Dartan, Mach, Srinivas, Timmer, Fleck and Hulskamp2008; Pesch & Hulskamp, Reference Pesch and Hulskamp2009). The complexity of protein interactions and intercellular mobility among trichome patterning proteins makes it challenging to analyse the relative contribution between these two models. However, using weak ttg1 alleles to understand the regulatory circuits of trichome patterning indicated that TTG1 severs a key component in both the activator–inhibitor and activator–depletion models (Balkunde et al., Reference Balkunde, Deneer, Bechtel, Zhang, Herberth, Pesch, Jaegle, Fleck and Hulskamp2020). The authors further determined that the core trichome patterning modules in both models differ in their activation of the long-range inhibitor CPC and the short-range inhibitor TRY (Balkunde et al., Reference Balkunde, Deneer, Bechtel, Zhang, Herberth, Pesch, Jaegle, Fleck and Hulskamp2020).

In contrast to the two models of trichome development, stomatal patterning relies on cell-to-cell signalling through secreted peptides. The inhibitory signalling peptide family EPF (Hara et al., Reference Hara, Kajita, Torii, Bergmann and Kakimoto2007; Reference Hara, Yokoo, Kajita, Onishi, Yahata, Peterson, Torii and Kakimoto2009; Hunt & Gray, Reference Hunt and Gray2009) and the activator peptide Stomagen (Sugano et al., Reference Sugano, Shimada, Imai, Okawa, Tamai, Mori and Hara-Nishimura2010) synergistically influence stomatal patterning. Using mosaic analysis and the computational pipeline SPACE (stomata patterning autocorrelation on epidermis), a recent study showed that both EPF1 and Stomagen have non-cell-autonomous effects, with EPF1 having a broader effective range (100–150 mm) than Stomagen (~60 mm) (Zeng et al., Reference Zeng, Lo, Hazelton, Morales and Torii2020). This spatial correlation with the effective range of small peptides provides information at a longer-range distance as opposed to the local information about the pattern.

The interplay of cell-to-cell signalling together with the regulatory circuit that controls stomatal initiation is the key to generating a pattern, in addition to the polarity-switch mechanism already mentioned. In a two-dimensional spatial patterning model of the stomatal lineage, the SCRM-SPCH complex forms a positive feedback loop that promotes the stomatal fate as well as the production of the secreted peptide EPF2 and the receptor modifier TMM, which in turn inhibits SPCH and SCRM. Thus, the resulting negative feedback loop reinforces the formation of a stomate according to the one-cell-spacing rule (Horst et al., Reference Horst, Fujita, Lee, Rychel, Garrick, Kawaguchi, Peterson and Torii2015). This work provided an example using an intrinsic molecular framework to generate a self-organising two-dimensional patterning of stomatal linage initiation (Horst et al., Reference Horst, Fujita, Lee, Rychel, Garrick, Kawaguchi, Peterson and Torii2015). After stomatal fate is determined, stomatal cells will undergo one round of symmetric cell division to produce a pair of guard cells. How do cells divide only once? Downstream targets of MUTE, consisting of a cell cycle regulator and its transcriptional repressor, were proposed to form a typical incoherent type I feed-forward loop to orchestrate and generate this single symmetric division event (Han et al., Reference Han, Qi, Sugihara, Dang, Endo, Miller, Kim, Miura and Torii2018).

4.3. Auxin

Auxin is a highly diffusible phytohormone that plays a crucial role in plant morphogenesis and growth by responding to intrinsic and external cues. The spatiotemporal distribution of auxin modulates the patterning and placement of cells and organs. Mathematical modelling has been used to precisely describe how auxin coordinates plant growth (Allen & Ptashnyk, Reference Allen and Ptashnyk2020; Smith et al., Reference Smith, Guyomarc'h, Mandel, Reinhardt, Kuhlemeier and Prusinkiewicz2006; van Berkel et al., Reference van Berkel, de Boer, Scheres and ten Tusscher2013). Since auxin gradients drive root architecture and tropic responses, previous studies have investigated the link between auxin and root development. Through cell-type-specific induction of auxin biosynthesis and morphokinetic analysis, Hu et al. (Reference Hu, Omary, Hu, Doron, Hoermayer, Chen, Megides, Chekli, Ding, Friml, Zhao, Tsarfaty and Shani2021) quantitatively analysed root growth and skewing and created a toolbox for studying auxin-mediated plant development at a single-cell level.

Auxin is also an important factor controlling leaf development. Pavement cells are often used to investigate non-transcriptional ABP1-TMK-mediated auxin signalling (Xu et al., Reference Xu, Dai, Chen, Nagawa, Cao, Li, Zhou, Chen, De Rycke, Rakusova, Wang, Jones, Friml, Patterson, Bleecker and Yang2014). Auxin initiates interdigitated growth in leaf pavement cells by controlling TMK1 and ROP signalling. TMK1 also facilitates the formation of flotillin1-associated ordered nanodomains at the plasma membrane, manages cortical microtubule organisation, and changes the shape of pavement cells (Pan et al., Reference Pan, Fang, Liu, Senay-Aras, Lin, Zheng, Zhang, Guo, Manor, Van Norman, Chen and Yang2020).

A survey of auxin dynamics during stomatal development established that auxin levels decreased in the small sister cell (meristemoid) after asymmetric cell division (Le et al., Reference Le, Liu, Yang, Chen, Zou, Wang, Wang, Vanneste, Morita, Tasaka, Ding, Friml, Beeckman and Sack2014). In one study, a fluctuating auxin gradient was observed in spirally formed pavement cells and was associated with the jigsaw-puzzle shape of pavement cells on the epidermis (Grones et al., Reference Grones, Majda, Doyle, Van Damme and Robert2020). This study used a synthetic auxin output reporter, DR5:Venus-NLS (with the DR5 promoter driving the expression of an expression cassette encoding the fluorescent protein Venus fused to a nuclear localization sequence [NLS]), to trace SLGC divisions. The authors detected an association between increased auxin output and spirals of SLGC divisions. Moreover, the outermost SLGC with a high auxin level tended to become a lobed cell (Grones et al., Reference Grones, Majda, Doyle, Van Damme and Robert2020). Because auxin orchestrates a mitotic-to-endocycle switch in Arabidopsis (Ishida et al., Reference Ishida, Adachi, Yoshimura, Shimizu, Umeda and Sugimoto2010), auxin may determine the transition from SLGCs to pavement cells.

Two additional auxin sensors, R2D2 (ratiometric version of two DIIs) (Brunoud et al., Reference Brunoud, Wells, Oliva, Larrieu, Mirabet, Burrow, Beeckman, Kepinski, Traas, Bennett and Vernoux2012; Liao et al., Reference Liao, Smet, Brunoud, Yoshida, Vernoux and Weijers2015) and the auxin biosensor AuxSen (Herud-Sikimic et al., Reference Herud-Sikimic, Stiel, Kolb, Shanmugaratnam, Berendzen, Feldhaus, Hocker and Jurgens2021), have been deployed to monitor auxin responses (R2D2) and concentrations (AuxSen) during development. The DII domain is the auxin-dependent degradation domain II of an Aux/IAA protein, so the fluorescence signal of DII-Venus decreases when auxin levels are high. A mutated DII domain (mDII) that is insensitive to auxin-mediated degradation can be used as a control for semi-quantitative measurements, whereby the mDII-ntdTomato/DII-Venus ratio is proportional to the levels of auxin signal transduction. The auxin biosensor uses an engineered tryptophan repressor from Escherichia coli for auxin sensing, and the readout is based on fluorescence resonance energy transfer signal (Herud-Sikimic et al., Reference Herud-Sikimic, Stiel, Kolb, Shanmugaratnam, Berendzen, Feldhaus, Hocker and Jurgens2021). This biosensor is effective in dynamically probing the actual concentration and location of auxin inside a cell. Further analysis of auxin responses in the epidermis may reveal the coordination of different cell types in epidermal formation.

4.4. Cell cycle

Many key transcription factors driving cell fate determination in the leaf epidermis have been identified using forward genetic screens. However, cell fate is not only controlled by transcription factors, but is also associated with specific cell cycle phases (Chen et al., Reference Chen, Hartman and Guo2015). Almost 30 years ago, a classic study showed that differentiation can be induced during the G1 phase in isolated pluripotent embryonal carcinoma cells, but not at any other cell cycle phase (Mummery et al., Reference Mummery, van den Brink and de Laat1987). Earlier studies on plant xylem cell differentiation had suggested that DNA synthesis was required (entering the S phase) before xylem cell differentiation, which was contradictory to the G1 phase observations. A model was proposed to resolve this apparent conflict by which cells in early G1 receive a signal and enter differentiation, whereas cells in late G1 need to go through all other phases (S, G2, and M) before reaching early G1 to differentiate (Dodds, Reference Dodds1981). A recent study showed that manipulating the duration of the G1 phase by overexpressing the CDK inhibitor gene SIAMESE-RELATED4 (SMR4) can reduce cell proliferation of the meristemoid (Han et al., Reference Han, Herrmann, Yang, Iwasaki, Sakamoto, Desvoyes, Kimura, Gutierrez, Kim and Torii2022).

During stomatal development, SLGCs can serve as a stem-cell-like pool to replenish stomatal precursors or differentiate into pavement cells. According to the transcriptomic signatures of SLGCs, proliferation and differentiation are regulated by both activators and repressors of mitosis and endocycles (Ho et al., Reference Ho, Bringmann, Oshima, Mitsuda and Bergmann2021), indicating a connection between cell fate and the cell cycle machinery. Low endoreplication levels can result in loss of trichome identity, with cells dedifferentiating into pavement cells (Bramsiepe et al., Reference Bramsiepe, Wester, Weinl, Roodbarkelari, Kasili, Larkin, Hülskamp and Schnittger2010). When endocycle inhibitors are genetically inactivated, endoreduplicated cells inappropriately evoke a guard cell identity (Iwata et al., Reference Iwata, Ikeda, Matsunaga, Kurata, Yoshioka, Criqui, Genschik and Ito2011). As with the leaf epidermis, the formation of giant cells in Arabidopsis sepals also requires a CDK inhibitor, LOSS OF GIANT CELLS FROM ORGANS (LOG), at the G2-to-M phase transition to produce endoreduplicated cells (Roeder et al., Reference Roeder, Chickarmane, Cunha, Obara, Manjunath and Meyerowitz2010). The ploidy level affects nuclear size, nuclear pore density, chromatin compaction, and the distance between transcription sites and nuclear pores (Robinson et al., Reference Robinson, Coate, Singh, Hong, Bush, Doyle and Roeder2018; Roeder et al., Reference Roeder, Otegui, Dixit, Anderson, Faulkner, Zhang, Harrison, Kirchhelle, Goshima, Coate, Doyle, Hamant, Sugimoto, Dolan, Meyer, Ehrhardt, Boudaoud and Messina2022). These factors may further affect chromatin accessibility and alter the transcriptional profile of cells.

Stomatal patterning is mediated by asymmetric cell division driven by SPCH and symmetric cell division driven by MUTE and FAMA. Using time-lapse imaging, Han et al. (Reference Han, Herrmann, Yang, Iwasaki, Sakamoto, Desvoyes, Kimura, Gutierrez, Kim and Torii2022) identified a longer cell cycle length in symmetric cell division compared to that of asymmetric cell division. Further analysis showed that the cell fate determinator MUTE directly upregulates the CDK inhibitor gene SMR4 to slow down the G1 phase and allow the transition to cell differentiation. During Arabidopsis sepal development, the pattern of giant cells is associated with the fluctuating concentration of the transcription factor ATML1 during the G2 phase (Meyer et al., Reference Meyer, Teles, Formosa-Jordan, Refahi, San-Bento, Ingram, Jönsson, Locke and Roeder2017). If ATML1 levels pass a threshold during the G2 phase, the cell will likely enter endoreduplication and become a giant cell. To probe and quantify the length of different cell cycle phases (e.g., G1, S, G2 and M), live-cell imaging tools have been developed such as Cell Cycle Tracking in Plant Cells (Cytrap) (Yin et al., Reference Yin, Ueda, Takagi, Kajihara, Sugamata Aki, Nobusawa, Umeda-Hara and Umeda2014) and plant cell cycle indicator (PlaCCI) (Desvoyes et al., Reference Desvoyes, Arana-Echarri, Barea and Gutierrez2020).

Cytrap is a dual-colour system with an S+G2 phase marker and a G2/M phase reporter (Yin et al., Reference Yin, Ueda, Takagi, Kajihara, Sugamata Aki, Nobusawa, Umeda-Hara and Umeda2014). Arabidopsis CDT1a functions in DNA replication origin licencing. Its C-terminal region is responsible for the proteasome-mediated degradation at the late G2 or early M phase. Therefore, the C terminus of CDT1a was fused to the red fluorescent protein (RFP), and the encoding expression cassette was driven by an S-specific promoter from HISTONE THREE RELATED2 (HTR2), a histone 3.1-type gene, to create the S+G2 reporter. Together with the G2/M phase-specific CYCB1-GFP marker (encoding a fusion between cyclin B1 and green fluorescent protein), this system allows the visualisation of both S-to-G2 and G2-to-M cell cycle stages. Since Cytrap uses GFP and RFP, the protein of interest can be fused to cyan fluorescent protein (CFP) to trace its dynamics during the cell cycle (Figure 3b).

In PlaCCI, CDT1a-CFP, HTR13-mCherry, and CYCB1;1-GFP are driven by their own promoters to identify G1, S + early G2, and late G2 + M (prophase and metaphase) phase cells, respectively (Desvoyes et al., Reference Desvoyes, Arana-Echarri, Barea and Gutierrez2020). All three reporters were integrated into a single transgene, thus facilitating transgenic plant production. Further analysis using these tools to identify different cell cycle phases and the parameters of cell size and shape should improve our understanding of the relationship between the cell cycle and cell fate determination (Figure 3b).

4.5. Cell division and cell size

Arabidopsis leaf development is driven by two processes: cell division and cell expansion (Green & Bauer, Reference Green and Bauer1977). Spatiotemporal leaf epidermal development exhibits a proximal zone of division competence and a distal zone with expansion capacity (Fox et al., Reference Fox, Southam, Pantin, Kennaway, Robinson, Castorina, Sanchez-Corrales, Sablowski, Chan, Grieneisen, Maree, Bangham and Coen2018). Analysing wild-type and spch mutant plants revealed the cell-autonomous function of SPCH in promoting division at smaller cell sizes and/or for shorter cell cycle length (Fox et al., Reference Fox, Southam, Pantin, Kennaway, Robinson, Castorina, Sanchez-Corrales, Sablowski, Chan, Grieneisen, Maree, Bangham and Coen2018). However, the growth rate was similar between wild-type and spch plants, suggesting that cell division is uncoupled from cell expansion (Fox et al., Reference Fox, Southam, Pantin, Kennaway, Robinson, Castorina, Sanchez-Corrales, Sablowski, Chan, Grieneisen, Maree, Bangham and Coen2018). A combination of time-lapse imaging of epidermal growth and modelling in wild-type plants also showed that the average cell cycle duration remained constant throughout epidermal development (Asl et al., Reference Asl, Dhondt, Boudolf, Beemster, Beeckman, Inze, Govaerts and De Veylder2011). No maximum cell size threshold was found for cell division during pavement cell formation, suggesting that the cell cycle rather than cell size controls cell division events (Asl et al., Reference Asl, Dhondt, Boudolf, Beemster, Beeckman, Inze, Govaerts and De Veylder2011). In SAM, a study showed that both G1/S and G2/M transitions are size-dependent, with larger cells exiting the G1 phase or entering the subsequent S phase more rapidly than smaller cells, thereby generating uniformly sized cells (Jones et al., Reference Jones, Forero-Vargas, Withers, Smith, Traas, Dewitte and Murray2017). The cell size checkpoint is not triggered by the G2/M phase for cell division in SAM, ruling out the models that cells undergo cell division at a fixed time after birth or there is a critical size increment between divisions (Willis et al., Reference Willis, Refahi, Wightman, Landrein, Teles, Huang, Meyerowitz and Jonsson2016). Rather, the observation showed that the cell size fluctuations decay by ~75% is intermediate between critical increment and critical size, suggesting a diluter mechanism may account for the cell size regulation (Willis et al., Reference Willis, Refahi, Wightman, Landrein, Teles, Huang, Meyerowitz and Jonsson2016). An asymmetric cell division dilution model then suggests that DNA acts as an internal scale for cell size (D’Ario et al., Reference D’Ario, Tavares, Schiessl, Desvoyes, Gutierrez, Howard and Sablowski2021). In this inhibitor dilution model, one of the cell cycle inhibitors, KRP4 (KIP-RELATED PROTEIN4), is more diluted in the larger cell after cell division. Therefore, the larger cell enters the cell cycle faster than the smaller cell. The observations from SAM formation and leaf epidermal development indicate the importance of cell cycle and asymmetric cell division in controlling cell size homeostasis in the complex environment of multicellular tissues. The SAM is a zone containing division-competent plant stem cells, while the leaf epidermis comprises hundreds of lineages at different stages of cell division and differentiation, thus making the leaf epidermis a more complex system.

In the context of a tissue, topology and geometry are two important aspects to consider, in addition to division rate, when studying the mechanisms underlying epidermal development. Geometry refers to cell shape and size, whereas topology refers to their connectivity within the tissue, for example, the number of neighbours each cell has (Carter et al., Reference Carter, Sánchez-Corrales, Hartley, Grieneisen and Marée2017). Surprisingly, the topological distribution for the entire cell population is identical between the epidermis of young and old leaves in spch plants, which do not have stomata (Carter et al., Reference Carter, Sánchez-Corrales, Hartley, Grieneisen and Marée2017). This finding suggested that the whole leaf maintains globally topological homoeostasis across developmental time and developmentally distinct zones such as proximal and distal regions (Carter et al., Reference Carter, Sánchez-Corrales, Hartley, Grieneisen and Marée2017). However, as the epidermis is made of different types of epidermal cells in plants, whether the cell type-specific growth locally shapes a tissue remains unclear. The comparison of the epidermal growth in WT and spch cotyledons indicates that stomatal differentiation through the lineage is the driving force for growth variability (Le Gloanec et al., Reference Le Gloanec, Collet, Silveira, Wang, Routier-Kierzkowska and Kierzkowski2022). Those local growth differences are buffered by the adjacent cells of stomata and trichomes to ensure reproducible development (Le Gloanec et al., Reference Le Gloanec, Collet, Silveira, Wang, Routier-Kierzkowska and Kierzkowski2022). Furthermore, to generate diverse leaf shapes, the combination and the arrangement of cell division and cell expansion need to be considered in different zones during leaf development. The molecular interplay between global differentiation across the entire leaf and the local patterning of growing foci along the margin are the keys to making a simple leaf or a dissected leaf in different species (Kierzkowski et al., Reference Kierzkowski, Runions, Vuolo, Strauss, Lymbouridou, Routier-Kierzkowska, Wilson-Sanchez, Jenke, Galinha, Mosca, Zhang, Canales, Dello Ioio, Huijser, Smith and Tsiantis2019).

Endoreduplication is a means to increasing DNA abundance in a single cell, and it is often associated with cell differentiation, as mature trichomes and pavement cells are polyploid in the leaf epidermis. Many studies have reported a positive correlation between DNA content and cell size during development (Melaragno et al., Reference Melaragno, Mehrotra and Coleman1993; Sugimoto-Shirasu & Roberts, Reference Sugimoto-Shirasu and Roberts2003). Therefore, the coordination of endoreduplication and cell size is crucial for organ morphogenesis. But how are these two phenomena related? Robinson et al. (Reference Robinson, Coate, Singh, Hong, Bush, Doyle and Roeder2018) used live-cell imaging and quantitative approaches to investigate the nuclear volume, cell size, cell number, and organ size in sepals of mutants bearing different levels of endopolyploidy or whole-genome ploidy levels (diploid, tetraploid and octoploid). In a perfect compensation model, organ size would remain the same when cell size increases but would be accompanied by fewer cells, such that the area of eight diploid cells would be equal that of two octoploid cells. However, empirical data showed that cell size generally scales up with organ size, although the magnitude of this effect is dampened by compensation, meaning that the cell size increases with ploidy levels but only to a point (Robinson et al., Reference Robinson, Coate, Singh, Hong, Bush, Doyle and Roeder2018). The scaling effect is also cell-type specific. For example, the size of pavement cells in sepals increases linearly while the size of sepal guard cells increases exponentially in response to elevated ploidy levels (Robinson et al., Reference Robinson, Coate, Singh, Hong, Bush, Doyle and Roeder2018). Compared to the inner layers of leaves, the leaf epidermis responds more strongly to changes in ploidy by increasing cell size (Katagiri et al., Reference Katagiri, Hasegawa, Fujikura, Hoshino, Matsunaga and Tsukaya2016). This effect may be due to the air spaces in the inner tissue layers beneath the epidermis; to maintain the surface intact, mechanical forces imposed by cell-to-cell adhesion may produce pavement cells of various sizes. Although cell size remains similar in a mutant with smaller nuclei like crowded nuclei1 (crwn1), it is possible that DNA copy number or components from the nucleus or the nuclear envelope sense the change in ploidy and ultimately affect cell size (Robinson et al., Reference Robinson, Coate, Singh, Hong, Bush, Doyle and Roeder2018). In contrast to sepal development, stomatal formation occurs heterogeneously on the leaf surface and is not synchronised during development, making stomatal density a proxy to probe the termination of cell division (or reduced division events). The observation that sepals with high ploidy levels terminate cell division sooner than sepals with lower ploidy levels is consistent with the reduction in stomatal density as ploidy increases (Robinson et al., Reference Robinson, Coate, Singh, Hong, Bush, Doyle and Roeder2018).

In summary, with the available tools to obtain quantitative measurements of cell properties and signal concentrations in a spatiotemporal manner, we can start to use modelling approaches to systemically understand the development and predict the output of biological systems, such as patterning and cell fates.

5. Future prospects

Leaf epidermal development includes the development of stomatal and trichome cells into a functional tissue in which either stomata or trichomes are well separated from each other. Biochemical signalling, polarity establishment, and growth tension are integrated into the formation of complicated patterns. Although we have a good understanding of stomatal and trichome formation from genetic studies, we still do not understand how these two cell types communicate during development. For instance, we do not understand what determines the differentiation of protoderm cells into stomata, trichomes, or pavement cells or what governs SLGCs to become pavement cells or go through another round of asymmetric cell division.

Development is a continuous process that results in a heterogeneous population. Quantitative biology provides the methods and tools to describe this heterogeneous state. The studies and tools presented here provide the foundation to characterising leaf epidermis phenotypes and quantifying cellular behaviour at a single-cell level. Utilising cell-specific measurements such as polarity level, cell cycle status, transcription factor dynamics, and cell geometry over time can help us link mechanistic descriptions to observed phenotypes. Combined with computational modelling, these cell-specific measurements can help us determine the potential flow of information to illustrate developmental trajectories or even predict cell behaviour. Using simulations, the transcriptional or translational levels of key factors, cell-type specialisation, and pattern formation have been modelled to understand the formation of the SAM and Arabidopsis sepals (Klawe et al., Reference Klawe, Stiehl, Bastian, Gaillochet, Lohmann and Marciniak-Czochra2020; Meyer et al., Reference Meyer, Teles, Formosa-Jordan, Refahi, San-Bento, Ingram, Jönsson, Locke and Roeder2017).

To better understand leaf epidermal development, we need to further investigate the coordination of different cell types during their development. For example, tracing the dynamics of stomatal and trichome markers in the early developmental stage could help reveal interactions and fluctuations of cell state transitions in protoderm cells. Although there is no pavement-cell-type-specific marker, quantitative biology can be used to describe the transition from one cell state to another. Phenotypes (e.g., auxin gradients and lobe formation) associated with pavement cell maturation can allow monitoring of transition states to a mature state using time-lapse imaging.

Fueled by the power of single-cell multiomics data, cell identity can be precisely defined by the quantitative and high-resolution integration of gene expression and protein abundance profiles. Recently, numerous studies have investigated transcriptional patterns during leaf epidermal development at single-cell resolution (Xia et al., Reference Xia, Sun, Li, Li, Zhao, Chen, Qin, Chen, Chen, Liu, Yin, Mu, Wang, Xu, Li, Yuan, Qiao, Hao, Wang, Xie, Xu, Liu, Li, Chen, Liu, Yin, Yang, Wang, Gu and Xu2022; Zhang et al., Reference Zhang, Chen and Wang2021). These data are useful for reconstructing gene regulatory networks and identifying novel genes involved in cell fate commitment (Liu et al., Reference Liu, Zhou, Guo, Li, Tian, Zhu, Wang, Wu, Zhang, Hu, Sun, Yan, Li, Li, Hu, Guo, Rochaix, Miao and Sun2020; Lopez-Anido et al., Reference Lopez-Anido, Vatén, Smoot, Sharma, Guo, Gong, Anleu Gil, Weimer and Bergmann2021). An analysis of unsupervised clustering of transcriptome and pseudo-time trajectories revealed the flexibility of cell states during leaf epidermis development (Lopez-Anido et al., Reference Lopez-Anido, Vatén, Smoot, Sharma, Guo, Gong, Anleu Gil, Weimer and Bergmann2021). Additionally, assigning a cell cycle stage to each cell identity revealed that cell cycle regulators may coordinate with cell differentiation (Lopez-Anido et al., Reference Lopez-Anido, Vatén, Smoot, Sharma, Guo, Gong, Anleu Gil, Weimer and Bergmann2021). However, fluctuations in individual cell states may make it difficult to determine cell fate. Indeed, cell state can change over time when facing different internal or external stimuli. A cell can acquire a stable cell identity with a diverse cell state or phenotype (Morris, Reference Morris2019). Hence, a dynamic system with precise parameters to describe genotype and phenotype is needed to comprehend fate determination.

There is also a need to integrate transdisciplinary resources to shed light on leaf epidermis development. The Plant Cell Atlas is an exciting community resource that integrates spatiotemporal information from the microscale to the nanoscale and describes the dynamic developmental states of plants (Rhee et al., Reference Rhee, Birnbaum and Ehrhardt2019). The quantitative methods and tools summarised here will be useful to delineate epidermal phenotypes and cellular dynamics in cell state transitions. We hope that by incorporating transcriptome, genetic, and signalling network analyses, we will be able to predict cell behaviour and improve our understanding of the fundamental principles governing cell fate and leaf epidermal development.

Acknowledgements

We thank the reviewers for their advice and Academia Sinica for the support.

Financial support

This work was supported by Academia Sinica (grant number AS-CDA-111-L01).

Conflict of interest

The authors declare none.

Authorship contributions

C.K., S.-L.Y., and C.-M.K.H. wrote the manuscript.

Data availability statement

Data sharing is not applicable to this article as no datasets were generated or analysed here.

References

Abe, M., Katsumata, H., Komeda, Y., & Takahashi, T. (2003). Regulation of shoot epidermal cell differentiation by a pair of homeodomain proteins in Arabidopsis. Development (Cambridge, England), 130, 635643.CrossRefGoogle ScholarPubMed
Abe, T., Thitamadee, S., & Hashimoto, T. (2004). Microtubule defects and cell morphogenesis in the lefty1lefty2 tubulin mutant of Arabidopsis thaliana. Plant and Cell Physiology, 45, 211220.CrossRefGoogle ScholarPubMed
Allen, H. R., & Ptashnyk, M. (2020). Mathematical modelling of auxin transport in plant tissues: Flux meets signalling and growth. Bulletin of Mathematical Biology, 82, 17.CrossRefGoogle ScholarPubMed
Altartouri, B., Bidhendi, A. J., Tani, T., Suzuki, J., Conrad, C., Chebli, Y., Liu, N., Karunakaran, C., Scarcelli, G., & Geitmann, A. (2019). Pectin chemistry and cellulose crystallinity govern pavement cell morphogenesis in a multi-step mechanism. Plant Physiology, 181, 127141.CrossRefGoogle Scholar
Asaoka, M., Ooe, M., Gunji, S., Milani, P., Runel, G., Horiguchi, G., Hamant, O., Sawa, S., Tsukaya, H., & Ferjani, A. (2021). Stem integrity in Arabidopsis thaliana requires a load-bearing epidermis. Development (Cambridge, England), 148, dev198028.CrossRefGoogle ScholarPubMed
Asl, L. K., Dhondt, S., Boudolf, V., Beemster, G. T., Beeckman, T., Inze, D., Govaerts, W., & De Veylder, L. (2011). Model-based analysis of Arabidopsis leaf epidermal cells reveals distinct division and expansion patterns for pavement and guard cells. Plant Physiology, 156, 21722183.Google ScholarPubMed
Balkunde, R., Deneer, A., Bechtel, H., Zhang, B. P., Herberth, S., Pesch, M., Jaegle, B., Fleck, C., & Hulskamp, M. (2020). Identification of the trichome patterning Core network using data from weak ttg1 alleles to constrain the model space. Cell Reports, 33, 108497.CrossRefGoogle ScholarPubMed
Bergmann, D. C., Lukowitz, W., & Somerville, C. R. (2004). Stomatal development and pattern controlled by a MAPKK kinase. Science, 304, 14941497.CrossRefGoogle ScholarPubMed
Bidhendi, A. J., Altartouri, B., Gosselin, F. P., & Geitmann, A. (2019). Mechanical stress initiates and sustains the morphogenesis of wavy leaf epidermal cells. Cell Reports, 28, 12371250.e1236.CrossRefGoogle ScholarPubMed
Biot, E., Cortizo, M., Burguet, J., Kiss, A., Oughou, M., Maugarny-Cales, A., Goncalves, B., Adroher, B., Andrey, P., Boudaoud, A., & Laufs, P. (2016). Multiscale quantification of morphodynamics: MorphoLeaf software for 2D shape analysis. Development (Cambridge, England), 143, 34173428.Google ScholarPubMed
Bouyer, D., Geier, F., Kragler, F., Schnittger, A., Pesch, M., Wester, K., Balkunde, R., Timmer, J., Fleck, C., & Hulskamp, M. (2008). Two-dimensional patterning by a trapping/depletion mechanism: The role of TTG1 and GL3 in Arabidopsis trichome formation. PLoS Biology, 6, 11661177.CrossRefGoogle ScholarPubMed
Bramsiepe, J., Wester, K., Weinl, C., Roodbarkelari, F., Kasili, R., Larkin, J. C., Hülskamp, M., & Schnittger, A. (2010). Endoreplication controls cell fate maintenance. PLoS Genetics, 6, e1000996.CrossRefGoogle ScholarPubMed
Bringmann, M., & Bergmann, D. C. (2017). Tissue-wide mechanical forces influence the polarity of stomatal stem cells in Arabidopsis. Current Biology : CB, 27, 877883.CrossRefGoogle ScholarPubMed
Brunoud, G., Wells, D. M., Oliva, M., Larrieu, A., Mirabet, V., Burrow, A. H., Beeckman, T., Kepinski, S., Traas, J., Bennett, M. J., & Vernoux, T. (2012). A novel sensor to map auxin response and distribution at high spatio-temporal resolution. Nature, 482, 103106.CrossRefGoogle ScholarPubMed
Bylesjo, M., Segura, V., Soolanayakanahally, R. Y., Rae, A. M., Trygg, J., Gustafsson, P., Jansson, S., & Street, N. R. (2008). LAMINA: A tool for rapid quantification of leaf size and shape parameters. BMC Plant Biology, 8, 82.CrossRefGoogle Scholar
Carter, R., Sánchez-Corrales, Y. E., Hartley, M., Grieneisen, V. A., & Marée, A. F. M. (2017). Pavement cells and the topology puzzle. Development (Cambridge, England), 144, 43864397.Google ScholarPubMed
Chen, X., Hartman, A., & Guo, S. (2015). Choosing cell fate through a dynamic cell cycle. Current Stem Cell Reports, 1, 129138.CrossRefGoogle ScholarPubMed
Clark, P. J., & Evans, F. C. (1954). Distance to nearest neighbor as a measure of spatial relationships in populations. Ecology, 35, 445453.CrossRefGoogle Scholar
Clark, S. E., Running, M. P., & Meyerowitz, E. M. (1993). Clavata1, a regulator of meristem and flower development in Arabidopsis. Development (Cambridge, England), 119, 397418.CrossRefGoogle ScholarPubMed
Clark, S. E., Running, M. P., & Meyerowitz, E. M. (1995). Clavata3 is a specific regulator of shoot and floral meristem development affecting the same processes as Clavata1. Development (Cambridge, England), 121, 20572067.CrossRefGoogle Scholar
D’Ario, M., Tavares, R., Schiessl, K., Desvoyes, B., Gutierrez, C., Howard, M., & Sablowski, R. (2021). Cell size controlled in plants using DNA content as an internal scale. Science, 372, 1176.CrossRefGoogle ScholarPubMed
de Reuille, P. B., Routier-Kierzkowska, A.-L., Kierzkowski, D., Bassel, G. W., Schüpbach, T., Tauriello, G., Bajpai, N., Strauss, S., Weber, A., Kiss, A., Burian, A., Hofhuis, H., Sapala, A., Lipowczan, M., Heimlicher, M. B., Robinson, S., Bayer, E. M., Basler, K., Koumoutsakos, P., … Smith, R. S. (2015). MorphoGraphX: A platform for quantifying morphogenesis in 4D. eLife, 4, e05864.CrossRefGoogle Scholar
Desvoyes, B., Arana-Echarri, A., Barea, M. D., & Gutierrez, C. (2020). A comprehensive fluorescent sensor for spatiotemporal cell cycle analysis in Arabidopsis. Nature Plants, 6, 13301334.CrossRefGoogle ScholarPubMed
Dhondt, S., Van Haerenborgh, D., Van Cauwenbergh, C., Merks, R. M. H., Philips, W., Beemster, G. T. S., & Inze, D. (2012). Quantitative analysis of venation patterns of Arabidopsis leaves by supervised image analysis. Plant Journal, 69, 553563.CrossRefGoogle ScholarPubMed
Digiuni, S., Schellmann, S., Geier, F., Greese, B., Pesch, M., Wester, K., Dartan, B., Mach, V., Srinivas, B. P., Timmer, J., Fleck, C., & Hulskamp, M. (2008). A competitive complex formation mechanism underlies trichome patterning on Arabidopsis leaves. Molecular Systems Biology, 4, 217.CrossRefGoogle ScholarPubMed
Dodds, J. H. (1981). Relationship of the cell cycle to xylem cell differentiation: A new model. Plant, Cell & Environment, 4, 145146.CrossRefGoogle Scholar
Dong, J., MacAlister, C. A., & Bergmann, D. C. (2009). BASL controls asymmetric cell division in Arabidopsis. Cell, 137, 13201330.CrossRefGoogle ScholarPubMed
Fetter, K. C., Eberhardt, S., Barclay, R. S., Wing, S., & Keller, S. R. (2019). StomataCounter: A neural network for automatic stomata identification and counting. New Phytologist, 223, 16711681.CrossRefGoogle ScholarPubMed
Fletcher, L. C., Brand, U., Running, M. P., Simon, R., & Meyerowitz, E. M. (1999). Signaling of cell fate decisions by CLAVATA3 in Arabidopsis shoot meristems. Science, 283, 19111914.CrossRefGoogle ScholarPubMed
Fox, S., Southam, P., Pantin, F., Kennaway, R., Robinson, S., Castorina, G., Sanchez-Corrales, Y. E., Sablowski, R., Chan, J., Grieneisen, V., Maree, A. F. M., Bangham, J. A., & Coen, E. (2018). Spatiotemporal coordination of cell division and growth during organ morphogenesis. PLoS Biology, 16, e2005952.CrossRefGoogle ScholarPubMed
Fu, Y., Xu, T., Zhu, L., Wen, M., & Yang, Z. (2009). A ROP GTPase signaling pathway controls cortical microtubule ordering and cell expansion in Arabidopsis. Current biology : CB, 19, 18271832.CrossRefGoogle ScholarPubMed
Gong, Y., Alassimone, J., Varnau, R., Sharma, N., Cheung, L. S., & Bergmann, D. C. (2021a). Tuning self-renewal in the Arabidopsis stomatal lineage by hormone and nutrient regulation of asymmetric cell division. eLife, 10, e63335.CrossRefGoogle ScholarPubMed
Gong, Y., Varnau, R., Wallner, E.-S., Acharya, R., Bergmann, D. C., & Cheung, L. S. (2021b). Quantitative and dynamic cell polarity tracking in plant cells. New Phytologist, 230, 867877.CrossRefGoogle ScholarPubMed
Gorelova, V., Sprakel, J., & Weijers, D. (2021). Plant cell polarity as the nexus of tissue mechanics and morphogenesis. Nature Plants, 7, 15481559.CrossRefGoogle ScholarPubMed
Green, P. B., & Bauer, K. (1977). Analysing the changing cell cycle. Journal of Theoretical Biology, 68, 299315.CrossRefGoogle ScholarPubMed
Greese, B., Hulskamp, M., & Fleck, C. (2014). Quantification of variability in trichome patterns. Frontiers in Plant Science, 5, 596.CrossRefGoogle ScholarPubMed
Grones, P., Majda, M., Doyle, S. M., Van Damme, D., & Robert, S. (2020). Fluctuating auxin response gradients determine pavement cell-shape acquisition. Proceedings of the National Academy of Sciences, 117, 16027.CrossRefGoogle ScholarPubMed
Gudesblat, G. E., Schneider-Pizoń, J., Betti, C., Mayerhofer, J., Vanhoutte, I., van Dongen, W., Boeren, S., Zhiponova, M., de Vries, S., Jonak, C., & Russinova, E. (2012). SPEECHLESS integrates brassinosteroid and stomata signalling pathways. Nature Cell Biology, 14, 548554.CrossRefGoogle ScholarPubMed
Guo, X. Y., Ding, X., & Dong, J. (2022). Dichotomy of the BSL phosphatase signaling spatially regulates MAPK components in stomatal fate determination. Nature Communications, 13, 2438.CrossRefGoogle ScholarPubMed
Guo, X. Y., & Dong, J. (2019). To divide or differentiate: It is about scaffolding. Trends in Plant Science, 24, 481484.CrossRefGoogle ScholarPubMed
Guo, X. Y., Park, C. H., Wang, Z. Y., Nickels, B. E., & Dong, J. (2021). A spatiotemporal molecular switch governs plant asymmetric cell division. Nature Plants 7, 667.CrossRefGoogle ScholarPubMed
Haas, K. T., Wightman, R., Meyerowitz, E. M., & Peaucelle, A. (2020). Pectin homogalacturonan nanofilament expansion drives morphogenesis in plant epidermal cells. Science, 367, 10031007.CrossRefGoogle ScholarPubMed
Han, S. K., Herrmann, A., Yang, J., Iwasaki, R., Sakamoto, T., Desvoyes, B., Kimura, S., Gutierrez, C., Kim, E. D., & Torii, K. U. (2022). Deceleration of the cell cycle underpins a switch from proliferative to terminal divisions in plant stomatal lineage. Developmental Cell, 57, 569582.e566.CrossRefGoogle ScholarPubMed
Han, S. K., Qi, X., Sugihara, K., Dang, J. H., Endo, T. A., Miller, K. L., Kim, E. D., Miura, T., & Torii, K. U. (2018). MUTE directly orchestrates cell-state switch and the single symmetric division to create stomata. Developmental Cell 45, 303315.e305.CrossRefGoogle ScholarPubMed
Handley, R., Ekbom, B., & Agren, J. (2005). Variation in trichome density and resistance against a specialist insect herbivore in natural populations of Arabidopsis thaliana. Ecological Entomology, 30, 284292.CrossRefGoogle Scholar
Hara, K., Kajita, R., Torii, K. U., Bergmann, D. C., & Kakimoto, T. (2007). The secretory peptide gene EPF1 enforces the stomatal one-cell-spacing rule. Genes & Development, 21, 17201725.CrossRefGoogle ScholarPubMed
Hara, K., Yokoo, T., Kajita, R., Onishi, T., Yahata, S., Peterson, K. M., Torii, K. U., & Kakimoto, T. (2009). Epidermal cell density is autoregulated via a secretory peptide, EPIDERMAL PATTERNING FACTOR 2 in Arabidopsis leaves. Plant & Cell Physiology, 50, 10191031.CrossRefGoogle Scholar
He, J. X., Gendron, J. M., Yang, Y., Li, J., & Wang, Z. Y. (2002). The GSK3-like kinase BIN2 phosphorylates and destabilizes BZR1, a positive regulator of the brassinosteroid signaling pathway in Arabidopsis. Proceedings of the National Academy of Sciences of the United States of America, 99, 1018510190.CrossRefGoogle ScholarPubMed
Herud-Sikimic, O., Stiel, A. C., Kolb, M., Shanmugaratnam, S., Berendzen, K. W., Feldhaus, C., Hocker, B., & Jurgens, G. (2021). A biosensor for the direct visualization of auxin. Nature, 592, 768772.CrossRefGoogle ScholarPubMed
Ho, C. M., Paciorek, T., Abrash, E., & Bergmann, D. C. (2016). Modulators of stomatal lineage signal transduction Alter membrane contact sites and reveal specialization among ERECTA kinases. Developmental Cell, 38, 345357.CrossRefGoogle ScholarPubMed
Ho, C.-M. K., Bringmann, M., Oshima, Y., Mitsuda, N., & Bergmann, D. C. (2021). Transcriptional profiling reveals signatures of latent developmental potential in Arabidopsis stomatal lineage ground cells. Proceedings of the National Academy of Sciences, 118, e2021682118.CrossRefGoogle ScholarPubMed
Horst, R. J., Fujita, H., Lee, J. S., Rychel, A. L., Garrick, J. M., Kawaguchi, M., Peterson, K. M., & Torii, K. U. (2015). Molecular framework of a regulatory circuit initiating two-dimensional spatial patterning of stomatal lineage. PLoS Genetics, 11, e1005374.CrossRefGoogle ScholarPubMed
Houbaert, A., Zhang, C., Tiwari, M., Wang, K., de Marcos Serrano, A., Savatin, D. V., Urs, M. J., Zhiponova, M. K., Gudesblat, G. E., Vanhoutte, I., Eeckhout, D., Boeren, S., Karimi, M., Betti, C., Jacobs, T., Fenoll, C., Mena, M., de Vries, S., De Jaeger, G., & Russinova, E. (2018). POLAR-guided signalling complex assembly and localization drive asymmetric cell division. Nature, 563, 574578.CrossRefGoogle ScholarPubMed
Hu, Y. J., Omary, M., Hu, Y., Doron, O., Hoermayer, L., Chen, Q. G., Megides, O., Chekli, O., Ding, Z. J., Friml, J., Zhao, Y. D., Tsarfaty, I., & Shani, E. (2021). Cell kinetics of auxin transport and activity in Arabidopsis root growth and skewing. Nature Communications, 12, 1657.CrossRefGoogle ScholarPubMed
Hunt, L., & Gray, J. E. (2009). The signaling peptide EPF2 controls asymmetric cell divisions during stomatal development. Current Biology : CB, 19, 864869.CrossRefGoogle ScholarPubMed
Ishida, T., Adachi, S., Yoshimura, M., Shimizu, K., Umeda, M., & Sugimoto, K. (2010). Auxin modulates the transition from the mitotic cycle to the endocycle in Arabidopsis. Development (Cambridge, England), 137, 6371.CrossRefGoogle Scholar
Iwata, E., Ikeda, S., Matsunaga, S., Kurata, M., Yoshioka, Y., Criqui, M. C., Genschik, P., & Ito, M. (2011). GIGAS CELL1, a novel negative regulator of the anaphase-promoting complex/cyclosome, is required for proper mitotic progression and CELL fate determination in Arabidopsis. The Plant Cell, 23, 43824393.CrossRefGoogle ScholarPubMed
Jones, A. R., Forero-Vargas, M., Withers, S. P., Smith, R. S., Traas, J., Dewitte, W., & Murray, J. A. H. (2017). Cell-size dependent progression of the cell cycle creates homeostasis and flexibility of plant cell size. Nature Communications, 8, 15060.CrossRefGoogle Scholar
Kanaoka, M. M., Pillitteri, L. J., Fujii, H., Yoshida, Y., Bogenschutz, N. L., Takabayashi, J., Zhu, J.-K., & Torii, K. U. (2008). SCREAM/ICE1 and SCREAM2 specify three cell-state transitional steps leading to arabidopsis stomatal differentiation. The Plant Cell, 20, 17751785.CrossRefGoogle ScholarPubMed
Katagiri, Y., Hasegawa, J., Fujikura, U., Hoshino, R., Matsunaga, S., & Tsukaya, H. (2016). The coordination of ploidy and cell size differs between cell layers in leaves. Development (Cambridge, England), 143, 11201125.Google ScholarPubMed
Kayes, J. M., & Clark, S. E. (1998). CLAVATA2, a regulator of meristem and organ development in Arabidopsis. Development (Cambridge, England), 125, 38433851.CrossRefGoogle ScholarPubMed
Kierzkowski, D., Runions, A., Vuolo, F., Strauss, S., Lymbouridou, R., Routier-Kierzkowska, A.L., Wilson-Sanchez, D., Jenke, H., Galinha, C., Mosca, G., Zhang, Z. J., Canales, C., Dello Ioio, R., Huijser, P., Smith, R. S., & Tsiantis, M. (2019). A growth-based framework for leaf shape development and diversity. Cell, 177, 1405.CrossRefGoogle ScholarPubMed
Kim, T. W., Guan, S., Sun, Y., Deng, Z., Tang, W., Shang, J. X., Sun, Y., Burlingame, A. L., & Wang, Z. Y. (2009). Brassinosteroid signal transduction from cell-surface receptor kinases to nuclear transcription factors. Nature Cell Biology, 11, 12541260.CrossRefGoogle ScholarPubMed
Kim, T.-W., Michniewicz, M., Bergmann, D. C., & Wang, Z.-Y. (2012). Brassinosteroid regulates stomatal development by GSK3-mediated inhibition of a MAPK pathway. Nature, 482, 419422.CrossRefGoogle ScholarPubMed
Klawe, F. Z., Stiehl, T., Bastian, P., Gaillochet, C., Lohmann, J. U., & Marciniak-Czochra, A. (2020). Mathematical modeling of plant cell fate transitions controlled by hormonal signals. PLoS Computational Biology, 16, e1007523.CrossRefGoogle ScholarPubMed
Kurata, T., Ishida, T., Kawabata-Awai, C., Noguchi, M., Hattori, S., Sano, R., Nagasaka, R., Tominaga, R., Koshino-Kimura, Y., Kato, T., Sato, S., Tabata, S., Okada, K., & Wada, T. (2005). Cell-to-cell movement of the CAPRICE protein in Arabidopsis root epidermal cell differentiation. Development (Cambridge, England), 132, 53875398.CrossRefGoogle ScholarPubMed
Kutschera, U., & Nikas, K. J. (2007). The epidermal-growth-control theory of stem elongation: An old and a new perspective. Journal of Plant Physiology, 164, 13951409.CrossRefGoogle ScholarPubMed
Lampard, G. R., Macalister, C. A., & Bergmann, D. C. (2008). Arabidopsis stomatal initiation is controlled by MAPK-mediated regulation of the bHLH SPEECHLESS. Science, 322, 11131116.CrossRefGoogle ScholarPubMed
Larson-Rabin, Z., Li, Z., Masson, P. H., & Day, C. D. (2009). FZR2/CCS52A1 expression is a determinant of endoreduplication and cell expansion in Arabidopsis. Plant Physiology, 149, 874884.CrossRefGoogle ScholarPubMed
Le Gloanec, C., Collet, L., Silveira, S. R., Wang, B. H., Routier-Kierzkowska, A. L., & Kierzkowski, D. (2022). Cell type-specific dynamics underlie cellular growth variability in plants. Development (Cambridge, England), 149, dev200783.CrossRefGoogle ScholarPubMed
Le, J., Liu, X. G., Yang, K. Z., Chen, X. L., Zou, J. J., Wang, H. Z., Wang, M., Vanneste, S., Morita, M., Tasaka, M., Ding, Z. J., Friml, J., Beeckman, T., & Sack, F. (2014). Auxin transport and activity regulate stomatal patterning and development. Nature Communications, 5, 3090.CrossRefGoogle ScholarPubMed
Lee, J. S., Kuroha, T., Hnilova, M., Khatayevich, D., Kanaoka, M. M., McAbee, J. M., Sarikaya, M., Tamerler, C., & Torii, K. U. (2012). Direct interaction of ligand-receptor pairs specifying stomatal patterning. Genes & Development, 26, 126136.CrossRefGoogle ScholarPubMed
Li, S., Li, L., Fan, W., Ma, S., Zhang, C., Kim, J. C., Wang, K., Russinova, E., Zhu, Y., & Zhou, Y. (2022). LeafNet: A tool for segmenting and quantifying stomata and pavement cells. The Plant Cell, 34, 11711188.CrossRefGoogle ScholarPubMed
Liao, C. Y., Smet, W., Brunoud, G., Yoshida, S., Vernoux, T., & Weijers, D. (2015). Reporters for sensitive and quantitative measurement of auxin response. Nature Methods, 12, 207210.CrossRefGoogle ScholarPubMed
Liu, C. C., Li, Y., Xu, L., Li, M. X., Wang, J. M., Yan, P., & He, N. A. P. (2021). Stomatal arrangement pattern: A new direction to explore plant adaptation and evolution. Frontiers in Plant Science, 12, 655255.CrossRefGoogle ScholarPubMed
Liu, Z. X., Zhou, Y. P., Guo, J. G., Li, J. A., Tian, Z. X., Zhu, Z. N., Wang, J. J., Wu, R., Zhang, B., Hu, Y. J., Sun, Y. J., Yan, S. G., Li, W. Q., Li, T., Hu, Y. H., Guo, C. X., Rochaix, J. D., Miao, Y. C., & Sun, X. W. (2020). Global dynamic molecular profiling of stomatal lineage cell development by single-cell RNA sequencing. Molecular Plant, 13, 11781193.CrossRefGoogle ScholarPubMed
Lopez-Anido, C. B., Vatén, A., Smoot, N. K., Sharma, N., Guo, V., Gong, Y., Anleu Gil, M. X., Weimer, A. K., & Bergmann, D. C. (2021). Single-cell resolution of lineage trajectories in the Arabidopsis stomatal lineage and developing leaf. Developmental Cell, 56, 10431055.e1044.CrossRefGoogle ScholarPubMed
Lu, S., Zhao, H., Des Marais, D. L., Parsons, E. P., Wen, X., Xu, X., Bangarusamy, D. K., Wang, G., Rowland, O., Juenger, T., Bressan, R. A., & Jenks, M. A. (2012). Arabidopsis ECERIFERUM9 involvement in cuticle formation and maintenance of plant water status. Plant Physiology, 159, 930944.CrossRefGoogle ScholarPubMed
MacAlister, C. A., Ohashi-Ito, K., & Bergmann, D. C. (2007). Transcription factor control of asymmetric cell divisions that establish the stomatal lineage. Nature, 445, 537540.CrossRefGoogle ScholarPubMed
Malivert, A., Hamant, O., & Ingram, G. (2018). The contribution of mechanosensing to epidermal cell fate specification. Current Opinion in Genetics & Development, 51, 5258.CrossRefGoogle ScholarPubMed
Mayer, K. F. X., Schoof, H., Haecker, A., Lenhard, M., Jurgens, G., & Laux, T. (1998). Role of WUSCHEL in regulating stem cell fate in the Arabidopsis shoot meristem. Cell, 95, 805815.CrossRefGoogle ScholarPubMed
Melaragno, J. E., Mehrotra, B., & Coleman, A. W. (1993). Relationship between Endopolyploidy and cell size in epidermal tissue of Arabidopsis. The Plant Cell, 5, 16611668.CrossRefGoogle ScholarPubMed
Meyer, H. M., Teles, J., Formosa-Jordan, P., Refahi, Y., San-Bento, R., Ingram, G., Jönsson, H., Locke, J. C. W., & Roeder, A. H. K. (2017). Fluctuations of the transcription factor ATML1 generate the pattern of giant cells in the Arabidopsis sepal. eLife, 6, e19131.CrossRefGoogle ScholarPubMed
Möller, B., Poeschl, Y., Plötner, R., & Bürstenbinder, K. (2017). PaCeQuant: A tool for high-throughput quantification of pavement cell shape characteristics. Plant Physiology, 175, 9981017.CrossRefGoogle ScholarPubMed
Morris, S. A. (2019). The evolving concept of cell identity in the single cell era. Development (Cambridge, England), 146, dev169748.CrossRefGoogle ScholarPubMed
Mummery, C. L., van den Brink, C. E., & de Laat, S. W. (1987). Commitment to differentiation induced by retinoic acid in P19 embryonal carcinoma cells is cell cycle dependent. Developmental Biology, 121, 1019.CrossRefGoogle ScholarPubMed
Muroyama, A., Gong, Y., & Bergmann, D. C. (2020 ) Opposing, polarity-driven nuclear migrations underpin asymmetric divisions to pattern Arabidopsis Stomata. Current Biology, 30, 44674475.e4464.CrossRefGoogle ScholarPubMed
Nagatoshi, Y., Mitsuda, N., Hayashi, M., Inoue, S., Okuma, E., Kubo, A., Murata, Y., Seo, M., Saji, H., Kinoshita, T., & Ohme-Takagi, M. (2016) GOLDEN 2-LIKE transcription factors for chloroplast development affect ozone tolerance through the regulation of stomatal movement. Proceedings of the National Academy of Sciences of the United States of America, 113, 42184223.CrossRefGoogle ScholarPubMed
Naulin, P. I., Valenzuela, G., & Estay, S. A. (2017). Size matters: Point pattern analysis biases the estimation of spatial properties of stomata distribution. The New Phytologist, 213, 19561960.CrossRefGoogle ScholarPubMed
Nowak, J., Eng, R. C., Matz, T., Waack, M., Persson, S., Sampathkumar, A., & Nikoloski, Z. (2021). A network-based framework for shape analysis enables accurate characterization of leaf epidermal cells. Nature Communications, 12, 458.CrossRefGoogle ScholarPubMed
Ohashi-Ito, K., & Bergmann, D. C. (2006). Arabidopsis FAMA controls the final proliferation/differentiation switch during stomatal development. The Plant Cell, 18, 24932505.CrossRefGoogle ScholarPubMed
Okamoto, S., Negishi, K., Toyama, Y., Ushijima, T., & Morohashi, K. (2020). Leaf Trichome distribution pattern in Arabidopsis reveals gene expression variation associated with environmental adaptation. Plants-Basel, 9, 909.CrossRefGoogle ScholarPubMed
Pan, X., Fang, L., Liu, J., Senay-Aras, B., Lin, W., Zheng, S., Zhang, T., Guo, J., Manor, U., Van Norman, J., Chen, W., & Yang, Z. (2020). Auxin-induced signaling protein nanoclustering contributes to cell polarity formation. Nature Communications, 11, 3914.CrossRefGoogle ScholarPubMed
Payne, C. T., Zhang, F., & Lloyd, A. M. (2000). GL3 encodes a bHLH protein that regulates trichome development in arabidopsis through interaction with GL1 and TTG1. Genetics, 156, 13491362.CrossRefGoogle ScholarPubMed
Pesch, M., & Hulskamp, M. (2009). One, two, three…Models for trichome patterning in Arabidopsis? Current Opinion in Plant Biology, 12, 587592.CrossRefGoogle Scholar
Pillitteri, L. J., Peterson, K. M., Horst, R. J., & Torii, K. U. (2011). Molecular profiling of stomatal Meristemoids reveals new component of asymmetric cell division and commonalities among stem cell populations in Arabidopsis. The Plant Cell, 23, 3260.CrossRefGoogle ScholarPubMed
Pillitteri, L. J., Sloan, D. B., Bogenschutz, N. L., & Torii, K. U. (2007). Termination of asymmetric cell division and differentiation of stomata. Nature, 445, 501505.CrossRefGoogle ScholarPubMed
Ramalho, J. J., Jones, V. A. S., Mutte, S., & Weijers, D. (2022). Pole position: How plant cells polarize along the axes. The Plant Cell, 34, 174192.CrossRefGoogle ScholarPubMed
Remmler, L., & Rolland-Lagan, A. G. (2012). Computational method for quantifying growth patterns at the Adaxial leaf surface in three dimensions. Plant Physiology, 159, 2739.CrossRefGoogle ScholarPubMed
Rerie, W. G., Feldmann, K. A., & Marks, M. D. (1994). The GLABRA2 gene encodes a homeo domain protein required for normal trichome development in Arabidopsis. Genes & Development, 8, 13881399.CrossRefGoogle ScholarPubMed
Rhee, S. Y., Birnbaum, K. D., & Ehrhardt, D. W. (2019). Towards building a plant cell atlas. Trends in Plant Science, 24, 303310.CrossRefGoogle ScholarPubMed
Robinson, D. O., Coate, J. E., Singh, A., Hong, L. L., Bush, M., Doyle, J. J., & Roeder, A. H. K. (2018). Ploidy and size at multiple scales in the Arabidopsis sepal. The Plant Cell, 30, 23082329.CrossRefGoogle ScholarPubMed
Robinson, S., de Reuille, P. B., Chan, J., Bergmann, D., Prusinkiewicz, P., & Coen, E. (2011). Generation of spatial patterns through cell polarity switching. Science, 333, 14361440.CrossRefGoogle ScholarPubMed
Roeder, A. H., Chickarmane, V., Cunha, A., Obara, B., Manjunath, B. S., & Meyerowitz, E. M. (2010). Variability in the control of cell division underlies sepal epidermal patterning in Arabidopsis thaliana. PLoS Biology, 8, e1000367.CrossRefGoogle ScholarPubMed
Roeder, A. H. K., Otegui, M. S., Dixit, R., Anderson, C. T., Faulkner, C., Zhang, Y., Harrison, M. J., Kirchhelle, C., Goshima, G., Coate, J. E., Doyle, J. J., Hamant, O., Sugimoto, K., Dolan, L., Meyer, H., Ehrhardt, D. W., Boudaoud, A., & Messina, C. (2022). Fifteen compelling open questions in plant cell biology. The Plant Cell, 34, 72102.CrossRefGoogle ScholarPubMed
Rolland-Lagan, A. G., Remmler, L., & Girard-Bock, C. (2014). Quantifying shape changes and tissue deformation in leaf development. Plant Physiology, 165, 496505.CrossRefGoogle ScholarPubMed
Roodbarkelari, F., Bramsiepe, J., Weinl, C., Marquardt, S., Novák, B., Jakoby, M. J., Lechner, E., Genschik, P., & Schnittger, A. (2010). CULLIN 4-RING FINGER-LIGASE plays a key role in the control of endoreplication cycles in Arabidopsis trichomes. Proceedings of the National Academy of Sciences, 107, 15275.CrossRefGoogle Scholar
Rowe, M. H., Dong, J., Weimer, A. K., & Bergmann, D. C. (2019). A plant-specific polarity module establishes cell fate asymmetry in the arabidopsis stomatal lineage. bioRxiv 614636. https://doi.org/614610.611101/614636 CrossRefGoogle Scholar
Sampathkumar, A., Krupinski, P., Wightman, R., Milani, P., Berquand, A., Boudaoud, A., Hamant, O., Jönsson, H., & Meyerowitz, E. M. (2014). Subcellular and supracellular mechanical stress prescribes cytoskeleton behavior in Arabidopsis cotyledon pavement cells. eLife, 3, e01967.CrossRefGoogle ScholarPubMed
Sanchez-Corrales, Y. E., Hartley, M., van Rooij, J., Maree, A. F. M., & Grieneisen, V. A. (2018). Morphometrics of complex cell shapes: Lobe contribution elliptic Fourier analysis (LOCO-EFA). Development (Cambridge, England), 145, dev156778.CrossRefGoogle ScholarPubMed
Sapala, A., Runions, A., Routier-Kierzkowska, A.-L., Das Gupta, M., Hong, L., Hofhuis, H., Verger, S., Mosca, G., Li, C.-B., Hay, A., Hamant, O., Roeder, A. H. K., Tsiantis, M., Prusinkiewicz, P., & Smith, R. S. (2018). Why plants make puzzle cells, and how their shape emerges. eLife, 7, e32794.CrossRefGoogle ScholarPubMed
Savaldi-Goldstein, S., Peto, C., & Chory, J. (2007). The epidermis both drives and restricts plant shoot growth. Nature, 446, 199202.CrossRefGoogle ScholarPubMed
Schellmann, S., Schnittger, A., Kirik, V., Wada, T., Okada, K., Beermann, A., Thumfahrt, J., Jurgens, G., & Hulskamp, M. (2002). TRIPTYCHON and CAPRICE mediate lateral inhibition during trichome and root hair patterning in Arabidopsis. The EMBO Journal, 21, 50365046.CrossRefGoogle ScholarPubMed
Schnittger, A., Folkers, U., Schwab, B., Jurgens, G., & Hulskamp, M. (1999). Generation of a spacing pattern: The role of TRIPTYCHON in trichome patterning in Arabidopsis. The Plant Cell, 11, 11051116.CrossRefGoogle ScholarPubMed
Schoof, H., Lenhard, M., Haecker, A., Mayer, K. F. X., Jurgens, G., & Laux, T. (2000). The stem cell population of Arabidopsis shoot meristems is maintained by a regulatory loop between the CLAVATA and WUSCHEL genes. Cell, 100, 635644.CrossRefGoogle ScholarPubMed
Shpak, E. D., McAbee, J. M., Pillitteri, L. J., & Torii, K. U. (2005). Stomatal patterning and differentiation by synergistic interactions of receptor kinases. Science, 309, 290293.CrossRefGoogle ScholarPubMed
Smith, R. S., Guyomarc'h, S., Mandel, T., Reinhardt, D., Kuhlemeier, C., & Prusinkiewicz, P. (2006). A plausible model of phyllotaxis. Proceedings of the National Academy of Sciences of the United States of America, 103, 13011306.CrossRefGoogle ScholarPubMed
Strauss, S., Runions, A., Lane, B., Eschweiler, D., Bajpai, N., Trozzi, N., Routier-Kierzkowska, A. L., Yoshida, S., da Silveira, S. R., Vijayan, A., Tofanelli, R., Majda, M., Echevin, E., Le Gloanec, C., Bertrand-Rakusova, H., Adibi, M., Schneitz, K., Bassel, G. W., Kierzkowski, D., … Smith, R. S. (2022). Using positional information to provide context for biological image analysis with MorphoGraphX 2.0. eLife, 11, e72601.CrossRefGoogle ScholarPubMed
Stringer, C., Wang, T., Michaelos, M., & Pachitariu, M. (2021). Cellpose: A generalist algorithm for cellular segmentation. Nature Methods, 18, 100106.CrossRefGoogle ScholarPubMed
Sugano, S. S., Shimada, T., Imai, Y., Okawa, K., Tamai, A., Mori, M., & Hara-Nishimura, I. (2010). Stomagen positively regulates stomatal density in Arabidopsis. Nature, 463, 241U130.CrossRefGoogle ScholarPubMed
Sugimoto-Shirasu, K., & Roberts, K. (2003). “Big it up”: Endoreduplication and cell-size control in plants. Current Opinion in Plant Biology, 6, 544553.CrossRefGoogle ScholarPubMed
Szymanski, D. B., Jilk, R. A., Pollock, S. M., & Marks, M. D. (1998). Control of GL2 expression in Arabidopsis leaves and trichomes. Development (Cambridge, England), 125, 11611171.CrossRefGoogle ScholarPubMed
Szymanski, D. B., Marks, M. D., & Wick, S. M. (1999). Organized F-actin is essential for normal trichome morphogenesis in Arabidopsis. The Plant Cell, 11, 23312347.CrossRefGoogle ScholarPubMed
Tian, J., Han, L. B., Feng, Z. D., Wang, G. D., Liu, W. W., Ma, Y. P., Yu, Y. J., & Kong, Z. S. (2015). Orchestration of microtubules and the actin cytoskeleton in trichome cell shape determination by a plant-unique kinesin. eLife, 4, e09351.CrossRefGoogle ScholarPubMed
Trinh, D. C., Alonso-Serra, J., Asaoka, M., Colin, L., Cortes, M., Malivert, A., Takatani, S., Zhao, F., Traas, J., Trehin, C., & Hamant, O. (2021). How mechanical forces shape plant organs. Current Biology, 31, R143R159.CrossRefGoogle ScholarPubMed
Tsai, M.-Y., Kuan, C., Guo, Z.-L., Yang, H.-A., Chung, K.-F., & Ho, C.-M. K. (2022). Stomatal clustering in begonia improves water use efficiency by modulating stomatal movement and leaf structure. Plant–Environment Interactions, 3, 141154.CrossRefGoogle ScholarPubMed
Vadde, B. V. L., Challa, K. R., & Nath, U. (2018). The TCP4 transcription factor regulates trichome cell differentiation by directly activating GLABROUS INFLORESCENCE STEMS in Arabidopsis thaliana. The Plant Journal, 93, 259269.CrossRefGoogle ScholarPubMed
van Berkel, K., de Boer, R. J., Scheres, B., & ten Tusscher, K. (2013). Polar auxin transport: Models and mechanisms. Development (Cambridge, England), 140, 22532268.CrossRefGoogle ScholarPubMed
Verger, S., Long, Y., Boudaoud, A., & Hamant, O. (2018). A tension-adhesion feedback loop in plant epidermis. eLife, 7, e34460.CrossRefGoogle ScholarPubMed
Vofely, R. V., Gallagher, J., Pisano, G. D., Bartlett, M., & Braybrook, S. A. (2019). Of puzzles and pavements: A quantitative exploration of leaf epidermal cell shape. New Phytologist, 221, 540552.CrossRefGoogle ScholarPubMed
Walker, J. D., Oppenheimer, D. G., Concienne, J., & Larkin, J. C. (2000). SIAMESE, a gene controlling the endoreduplication cell cycle in Arabidopsis thaliana trichomes. Development (Cambridge, England), 127, 39313940.CrossRefGoogle ScholarPubMed
Wester, K., Digiuni, S., Geier, F., Timmer, J., Fleck, C., & Hulskamp, M. (2009). Functional diversity of R3 single-repeat genes in trichome development. Development (Cambridge, England), 136, 14871496.CrossRefGoogle ScholarPubMed
Willis, L., Refahi, Y., Wightman, R., Landrein, B., Teles, J., Huang, K. C., Meyerowitz, E. M., & Jonsson, H. (2016). Cell size and growth regulation in the Arabidopsis thaliana apical stem cell niche. Proceedings of the National Academy of Sciences of the United States of America, 113, E8238E8246.Google ScholarPubMed
Wolny, A., Cerrone, L., Vijayan, A., Tofanelli, R., Barro, A. V., Louveaux, M., Wenzl, C., Strauss, S., Wilson-Sanchez, D., Lymbouridou, R., Steigleder, S. S., Pape, C., Bailoni, A., Duran-Nebreda, S., Bassel, G. W., Lohmann, J. U., Tsiantis, M., Hamprecht, F. A., Schneitz, K., … Kreshuk, A. (2020). Accurate and versatile 3D segmentation of plant tissues at cellular resolution. eLife, 9, e57613.CrossRefGoogle ScholarPubMed
Wu, T. C., Belteton, S. A., Pack, J., Szymanski, D. B., & Umulis, D. M. (2016). LobeFinder: A convex Hull-based method for quantitative boundary analyses of lobed plant cells. Plant Physiology, 171, 23312342.CrossRefGoogle ScholarPubMed
Xia, K., Sun, H. X., Li, J., Li, J., Zhao, Y., Chen, L., Qin, C., Chen, R., Chen, Z., Liu, G., Yin, R., Mu, B., Wang, X., Xu, M., Li, X., Yuan, P., Qiao, Y., Hao, S., Wang, J., Xie, Q., Xu, J., Liu, S., Li, Y., Chen, A., Liu, L., Yin, Y., Yang, H., Wang, J., Gu, Y., & Xu, X. (2022). The single-cell stereo-seq reveals region-specific cell subtypes and transcriptome profiling in Arabidopsis leaves. Developmental Cell 57, 12991310 e1294.CrossRefGoogle ScholarPubMed
Xu, T., Dai, N., Chen, J., Nagawa, S., Cao, M., Li, H., Zhou, Z., Chen, X., De Rycke, R., Rakusova, H., Wang, W., Jones, A. M., Friml, J., Patterson, S. E., Bleecker, A. B., & Yang, Z. (2014). Cell surface ABP1-TMK auxin-sensing complex activates ROP GTPase signaling. Science, 343, 10251028.CrossRefGoogle ScholarPubMed
Xu, T., Wen, M., Nagawa, S., Fu, Y., Chen, J. G., Wu, M. J., Perrot-Rechenmann, C., Friml, J., Jones, A. M., & Yang, Z. (2010). Cell surface- and rho GTPase-based auxin signaling controls cellular interdigitation in Arabidopsis. Cell, 143, 99110.CrossRefGoogle ScholarPubMed
Yang, S. L., Tran, N., Tsai, M. Y., & Ho, C. K. (2022). Misregulation of MYB16 expression causes stomatal cluster formation by disrupting polarity during asymmetric cell divisions. The Plant Cell, 34, 455476.CrossRefGoogle ScholarPubMed
Yin, K., Ueda, M., Takagi, H., Kajihara, T., Sugamata Aki, S., Nobusawa, T., Umeda-Hara, C., & Umeda, M. (2014). A dual-color marker system for in vivo visualization of cell cycle progression in Arabidopsis. The Plant Journal, 80, 541552.CrossRefGoogle ScholarPubMed
Zeng, S. M., Lo, E. K. W., Hazelton, B. J., Morales, M. F., & Torii, K. U. (2020). Effective range of non-cell autonomous activator and inhibitor peptides specifying plant stomatal patterning. Development (Cambridge, England), 147, dev192237.CrossRefGoogle ScholarPubMed
Zhang, T.-Q., Chen, Y., & Wang, J.-W. (2021). A single-cell analysis of the Arabidopsis vegetative shoot apex. Developmental Cell, 56, 10561074.e1058.CrossRefGoogle ScholarPubMed
Zhang, X. G., Grey, P. H., Krishnakumar, S., & Oppenheimer, D. G. (2005). The IRREGULAR TRICHOME BRANCH loci regulate trichome elongation in Arabidopsis. Plant and Cell Physiology, 46, 15491560.CrossRefGoogle ScholarPubMed
Zhang, X. G., & Oppenheimer, D. G. (2004). A simple and efficient method for isolating trichomes for downstream analyses. Plant and Cell Physiology, 45, 221224.CrossRefGoogle ScholarPubMed
Zhang, Y., Wang, P., Shao, W., Zhu, J. K., & Dong, J. (2015). The BASL polarity protein controls a MAPK signaling feedback loop in asymmetric cell division. Developmental Cell, 33, 136149.CrossRefGoogle ScholarPubMed
Zhang, Z. J., Runions, A., Mentink, R. A., Kierzkowski, D., Karady, M., Hashemi, B., Huijser, P., Strauss, S., Gan, X. C., Ljung, K., & Tsiantis, M. (2020). A WOX/auxin biosynthesis module controls growth to shape leaf form. Current Biology, 30, 4857.CrossRefGoogle ScholarPubMed
Zhao, M., Morohashi, K., Hatlestad, G., Grotewold, E., & Lloyd, A. (2008). The TTG1-bHLH-MYB complex controls trichome cell fate and patterning through direct targeting of regulatory loci. Development (Cambridge, England), 135, 19911999.CrossRefGoogle ScholarPubMed
Zuch, D. T., Doyle, S. M., Majda, M., Smith, R. S., Robert, S., & Torii, K. U. (2022). Cell biology of the leaf epidermis: Fate specification, morphogenesis, and coordination. The Plant Cell, 34, 209227.CrossRefGoogle ScholarPubMed
Figure 0

Fig. 1. Key factors involved in fate determination and leaf epidermal patterning during development. (A) Three trajectories describe the three distinct cell types of the leaf epidermis. The development and size of the shoot apical meristem (SAM) is controlled by the CLAVATA3 (CLV3)-WUSCHEL (WUS)-mediated negative feedback loop. The transcription factor (TF) genes ARABIDOPSIS THALIANA MERISTEM LAYER1 (ATML1) and PROTODERMAL FACTOR2 (PDF2) are expressed in the outermost layer (L1, blue) in the SAM to establish epidermal cell identity. Cells in the L1 layer called protoderms give rise to trichome-initiating cells (yellow), meristemoid mother cells (light blue), and pavement cells (grey). During trichome development, the major TF, GLABRA2 (GL2), drives cells to become polyploid trichome cells; the differentiation state is maintained by endoreduplication. To form a stomate, the master TF, SPEECHLESS (SPCH), initiates asymmetric cell division in a meristemoid mother cell to generate a small meristemoid (green) and a stomatal lineage ground cell (SLGC, white). MUTE then replaces SPCH and commits the cell to becoming a guard mother cell. Subsequently, FAMA in the guard mother cell drives symmetric cell division, resulting in a pair of guard cells. An SLGC can either undergo differentiation to become a pavement cell or divide asymmetrically again to produce another stomate (labelled by a dashed line). To date, no cell-type-specific driving factors have been associated with pavement cell formation. However, pavement cell maturation is often coupled with endoreduplication. (B) The cell–cell communication between trichome and non-trichrome cells relies on TRIPTYCHON (TRY). Before trichome initiation, GL1, GL3, and TRANSPARENT TESTA GLABRA1 (TTG1) form a stable MBW complex to activate GL2 transcription. GL2 accumulation promotes trichome cell fate. Besides GL2, the MBW complex also activates TRY expression in trichome cells. TRY tends to move to the neighbouring non-trichome cell to replace GL1 and disrupt the formation of the MBW complex, thus repressing GL2 and inhibiting the trichome cell fate. (C) Stomatal patterning follows the one-cell-spacing rule, meaning that two stomata never directly contact each other, and this signalling is mediated through peptide-mediated inhibitory signals and polarity establishment during stomatal development. SPCH drives the accumulation of a signalling peptide, EPIDERMAL PATTERNING FACTOR2 (EPF2), in meristemoids. The secreted peptides then bind to members of the receptor-like kinase ERECTA family and the receptor-like protein TMM on the surface of neighbouring cells. The binding triggers a MAPK cascade that phosphorylates and inhibits SPCH activity, thus preventing stomatal fate in these neighbouring cells. The interplay of chemical transduction and the polarity complex consisting of BASL, BREVIS RADIX-LIKE2 (BRXL2), and POLAR is required for asymmetric cell division and serves as a scaffold for recruiting and exerting inhibitory signalling in non-stomatal lineage cells. (D) Pavement cell formation is controlled biochemically by auxin. The high auxin concentration at the lobe initiation site induces the asymmetric accumulation of RHO-RELATED PROTEIN FROM PLANTS (ROP)-ROP-INTERACTIVE CRIB MOTIF-CONTAINING PROTEIN (RIC) in the two pavement cells. For the lobing cell (left), the recruitment of ROP2 and RIC4 helps the formation of actin filaments (F-actin) and further results in the protrusion of the cell. For the indented cell (right), ROP6 and RIC1 stabilise microtubule organisation under parallel direction and further pull the cell, forming an indentation.

Figure 1

Table 1 Quantitative tools to measure leaf epidermis features

Figure 2

Fig. 2. Quantitative methods to describe leaf morphology and the different types of epidermal cells. (A) Leaf shape can be described by its length, width, and the length/width ratio. Circularity calculated by (4$\pi$×leaf area)/(square perimeter) indicates that the leaf shape is approximately round (circularity = 1) or contains serrations (circularity closer to 0). If serrations are visible on a leaf, the indent length and width can be used to describe the extent of serration. (B) Trichome phenotypes can be measured by the number of trichomes on a leaf and trichome morphology. Trichome density can be scored over an entire leaf or a given area. Trichome index is the number of trichomes divided by the number of total epidermal cells including trichome, stomatal, and pavement cells over a given area. The trichome stalk, the branching number, and the branching points can be used to represent trichome shape. The trichome branching index represents the average number of branches in a trichome population. (C) Stomatal phenotypes can be described by stomatal number, pattern, and dynamics. Stomatal density represents the number of stomata over a given area. The stomatal index is defined as the number of stomata divided by the total number of epidermal cells. Stomatal groups are the number of stomatal islands in a given area. Adjacent stomata are defined as one group. A cluster event represents the number of islands with adjacent stomata. Cluster frequency represents the error rate of forming stomatal clusters. The movements of stomata can be described by stomatal length and width. Pore length and width excluding guard cells may also be used. During stomatal opening, the stomatal and pore lengths decrease, while the pore width increases. (D) Pavement cell phenotypes can be described according to their shape including the parameters of area, perimeter, length and width. The aspect ratio calculates the ratio between cell length and width. The jigsaw-puzzle shape can be described by the number of lobes and indentations, which can be expressed as circularity, solidity, and completeness. Circularity is calculated as (4$\pi$×cell area)/(square perimeter). Solidity is the ratio between cell area and convex hull area. Completeness is the ratio between visible and total possible links. A visible link represents the link between two nodes without crossing over the cell outline. An invisible link is defined as a link between two nodes that crosses over the cell outline. All three parameters have maxima equal to 1. They decrease when the cell takes on the shape of a jigsaw-puzzle piece.

Figure 3

Fig. 3. Quantitative tools for measuring polarity and the cell cycle. (A) Polarity measurements. (i) The polarity degree is calculated by the crescent length (green) relative to the cell perimeter (green+pink). M: meristemoid. SLGC, stomatal lineage ground cell. (ii) Workflow for Polarity Measurement (POME), a Fiji-based semi-automated pipeline for polarity quantification: First, a line of 0° to 180° angle is defined by the centroid to the centre of polar protein mass. Second, the cell outline is reconstructed and visualised by quantification of the fluorescence intensity. Third, standard deviation (SD,$\sigma$), amplitude ($\alpha$), and baseline intensity ($\beta$) derived from the fluorescence intensity through Gaussian fitting quantify the degree of polarisation in the plasma membrane, with higher SD values representing higher polarity levels. (iii) Tissue-wide polarity orientation can be indicated by the angle (α) between the leaf midrib and the connection between the cell centroid (orange dot) and the midpoint of the polarity crescent. (B) Cell cycle measurements. (i) Cytrap (Cell cycle tracking in plant cells) line. The dual-colour cell cycle reporter line uses HTR2pro:CDT1a-RFP and CYCB1pro:CYCB1-GFP to indicate S/G2 and G2/M, respectively. (ii) PlaCCI (Plant Cell Cycle Indicator) line. The three-colour cell cycle reporter line adopted CDT1apro:CDT1a-CFP, CYCB1:1pro:CYCB1;1-YFP, and HTR13pro:HTR13-mCherry to indicate G1, G2/M, and the entire cell cycle, respectively.

Author comment: Using quantitative methods to understand leaf epidermal development — R0/PR1

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Review: Using quantitative methods to understand leaf epidermal development — R0/PR2

Conflict of interest statement

The last author Kimmy Ho and I were post-docs together in Dominique Bergmann’s lab at Stanford. Therefore, I had my PhD student Roxane Spiegelhalder review this manuscript together with me. So if you could acknowledge her on Publons as well, this would be highly appreciated!.

Comments

Comments to Author: This review written by Chi Kuan, Shao-Li Yang and Chin-Min Ho concisely discusses the formation of Arabidopsis thaliana epidermal cell types and gives a broad summary of quantitative methods used to describe leaf and epidermal cell fate parameters.

This review is well structured into several paragraphs, describing the formation of different epidermal cell types, and then discussing the quantitative methods generally used in leaf studies, here again, the authors focus on the leaf as a whole and the previously described epidermal cell types: pavement cells, stomata and trichomes.

Next, the authors list examples for several selected parameters such as the quantitative measurement of polarity, cell cycle, signals in general and auxin in particular and cell size, all described in their role in cell fate determination of epidermal cells with a focus on measurable parameters.

The discussed topic is summed up in the last part where the authors also give a future prospect on the quickly emerging field.

The text is accompanied by 3 aesthetically pleasing and very concise figures that summarize the key factors guiding the developmental trajectory of the leaf epidermis cell types on a general cell fate as well as a molecular level, illustrate the quantitative methods used to describe leaf morphology and parameters to describe the different epidermal cell types, and describe quantitative tools for measuring polarity and cell cycle. Additionally, all computational tools are listed in a well-structured table, classified by structure analyzed and handily supplied with the publication describing the tool as well as further detailed information on usage.

Overall this review is not only very well written and accompanied by beautiful and comprehensive figures and graphical abstract but can serve as a useful overview of a collection of methods for quantitative analysis of plant epidermal development.

One small general point I would like to address is that in the main part of the text when summarising the biological processes before listing the quantitative methods, the authors could indicate the transition between the two things a bit more distinctly as it is done e.g. in the auxin paragraph but e.g. a bit less in the polarity paragraph.

Specific minor suggestions are listed below that could improve the manuscript:

L76: elaborate or rephrase “to function”

L87: add comma “cells, possessing [...] shape, are associated..”

L261-262: stoma and stomate are used as singular for stomata. Consider using consistent form (suggested: stoma). see also L779, L785

L268: rephrase

279: BASL is also a polarly localized protein. rephrase

L451: typo “used to monitor a transition state”

L453: single-cell omics data

L795 L804: consider keeping the figure legend consistent. in A and B the legend title was a full sentence

L850: the tool is called POME not POEM according to Gong et al. 2021 (see also L870)

Review: Using quantitative methods to understand leaf epidermal development — R0/PR3

Conflict of interest statement

“Reviewer declares none”.

Comments

Comments to Author: The manuscript by Kuan et al reviews the current understanding of the formation of the Arabidopsis leaf epidermis as well as the quantitative tools that have been used to characterise it. The manuscript is well written, nicely structured and easy to read, and would be of interest to the readership of the Quantitative Plant Biology Journal. Yet, there are some points I would like to comment on, most importantly related to expanding and covering some further relevant literature in the field;

Major:

- Although the authors comment on modelling aspects during the text, there are some other modelling papers that have helped in understanding the regulatory network and patterning aspects in trichomes and in stomata. Even if they are not mentioned it detail, it would be good the readership is aware about this literature. Including some of these papers might require an update of the figures. For instance,

For the trichome side, I would suggest to mention: one of the earlier papers or reviews that mention the Activitor-Inhibitor and Activator-Depletion Model, eg Pesch and Hülskamp 2009 Curr Op Plant Biol, and Balkunde et al 2020 Cell Reports, which is a recent paper proposing how a more updated version of the regulatory network might be operating.

For the stomatal side, it would be also good to mention: Robinson et al 2011 Science, Horst et al 2015 Plos Genetics, and perhaps Han et al 2018 Dev Cell.

I am not necessarily asking to have a modelling section, although the authors could decide to do so, but rather to acknowlegde some of these references given they have been important for understanding cell fate decision making and the regulatory network in the leaf.

- The review is more focused in some parts to stomata, which is totally fine, but in some parts one would expect to have more references to trichomes or more generally to the leaf epidermis. This happens more clearly in the ‘signals’ section.

-I would suggest to expand more on the cell size and division and include some relevant papers such as Fox et al (2018) Plos Biol, Carter et al (2017) Development, Kierkowski et al (2019) Cell, Kheibarshekan Asl et al (2011) Plant Physiol.

Minor:

• I am aware it is difficult to cover all the relevant literature in this field, so I would suggest to have a disclaimer in the manuscript in which you say you will just cover part of it. If there are relevant specific topics related to quantitative aspects in the leaf epidermis that you are not covering, I would encourage to state it in the manuscript.

• About the patterning analysis, consider to add Naulin et al 2017 New Phytologist, the recent prespective paper by Liu et al (2020) in Front Plant Sci and also other references focusing more on pattern variability such as Greese et al 2014 Frontiers in Plant Sci.

• About the single cell RNAseq, there are two recent references I would ask to mention, Zhang et al 2021 Dev Cell and Xia et al 2022 Dev cell.

• When talking about cell size and ploidy, I would suggest to comment on Robinson et al 2018 The Plant Cell (note that this is in sepal).

• When referring to MGX, it would be better that, instead of pointing to their video tutorial, the MGX 2.0 paper is cited (see Strauss et al 2022 elife). Also, in my understanding, MGX 2.0 can use now deep learning for segmentation as well, but the cell classification as you mentioned is through an SVM classifier, which is a supervised machine learning tool, but does not rely on a neural network (so it would not be deep learning). As explained in Strauss et al, the authors could comment that shape morphology and positional information can be used for cell type classification.

• I would suggest that there is an explanatory caption associated to Table 1.

• PlaCCi is introduced twice, see lines 341 and 352.

• There are some typos, and although the article is nicely written, there are some sentences that might have some grammatical mistakes.

Recommendation: Using quantitative methods to understand leaf epidermal development — R0/PR4

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Decision: Using quantitative methods to understand leaf epidermal development — R0/PR5

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Author comment: Using quantitative methods to understand leaf epidermal development — R1/PR6

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Review: Using quantitative methods to understand leaf epidermal development — R1/PR7

Conflict of interest statement

Reviewer declares none.

Comments

Comments to Author: All our concerns were appropriately addressed.

Review: Using quantitative methods to understand leaf epidermal development — R1/PR8

Conflict of interest statement

“Reviewer declares none”.

Comments

Comments to Author: I appreciate the efforts made by the authors in addressing my comments, the manuscript now has been significantly improved. However, I have some additional minor comments and suggestions I would like the authors to consider. Please find them below:

(The authors might find be a few suggestions that I could have raised in the first round of revision, but I might have missed; if this is the case, I am sorry about it, but I hope such suggestions help in the improvement of the manuscript.)

-Although I appreciate the importance of the first new included section entitled ‘the epidermis as a lod-bearing layer for organ morphogenesis’, I am wondering whether the authors expand too much on it, and the focus of the review, which should be on quantitative methods to understand leaf epidermal development, is a bit more diluted with too many biological details. A possibility to fix it would be to shorten that section (or place part of it elsewhere in the text), such the reader gets more directed to the core of the quantitative aspects in the review.

-Although in the text asymmetric cell divisions in the stomatal lineage are mentioned, perhaps it might be worth emphazising in Section 2.2 that there can be several rounds of such divisions, which will impact on the resulting final pattern (Gong et al 2021, eLife).

-When describing the shape of pavement cells, it would be worth also mentioning the work by Y.E. Sanchez-Corrales (2018) in Development.

-Lines 215-217, please rephrase "“Trichomes can be described using the following parameters: cell proportion on the leaf epidermis, parameters for individual trichome cells, and trichome patterns (distribution). “

One possible rephrasing option is as follows:

“The presence of trichomes in the epidermis, their individual shape and their spatial organization can be described using different sets of parameters.”

-Line 237, please rephrase “ trichome patterning is a critical parameter ”, given trichome patterning is not a parameter

-Line 242, I suggest to change “using the nearest neighbor distance (NND) (Okamoto et al., 2020). ” by

“using the nearest neighbor distance (NND) between trichomes (Okamoto et al., 2020), where each individual trichome is considered as a point, what we will refer as the point-pattern approximation.” so the point-pattern analysis is introduced here and hot in lines 256-258)

-Line 248, I would also add that in the review by Greese at al they review several methods using the point pattern approximation, comparing experimental data and simulations. For consistency with the stomatal section afterwards, it might be good to mention a bit more here the point pattern analysis.

-Line 249, variation-> variability, to be consistent.

-Line 256, “In this point-pattern analysis,” I would add something like “similar to the described analysis in trichomes”, given I suggest the point-pattern is introduced earlier.

-Paragraph starting with line 267: I would suggest to take out the numbers (1), (2), (3), etc. Also, it might be good to expand that paragraph a bit more and comment on stomatal observables found in other publications such as Liu et al.

-Line 282, I would suggest to use another connector instead of ‘in addition to stomatal morphology’, given the previous paragraphs describe more than ‘stomatal morphology’. Note also that durint the text, ‘in addition’ is used many times, so consider using other connectors.

-Line 322, I would suggest to find a smoother transition to the time-laspe tracking section in section 3.5, rather than straightly discribing StomataCounter.

-Line 332, I would rephrase into something like ‘(…) and PlantSeg (Wolny et al. 2020) allow performing 3D cell segmentation and extract quantitative measures at the single cell level’, to avoid confusion, given that PlantSeg does not allow the selection of cells, but its segmentation.

-Paragraph starting with line 438. It might be worth emphasising a bit more that in Zeng et al (2020) they use quantitative measures that provide information at a longer range distances, as opposed to the NND, which provides more local information about the pattern (and/or also you could consider to bring this point up in section 3.3).

-448-449 I would suggest slightly change the start the paragraph, such that it is more connected to the previous one. Perhaps a slight rephrase such as:

“The interplay of cell-to-cell signalling together with the regulatory circuit controlling stomatal initiation is key in generating a pattern, in addition to the polarity-switch mechanism already mentioned”

-In the new section referring to cell division, current models of cell division in the meristem are mentioned, so I would also suggest to mention Willis et al 2016 in PNAS.

-Lines 591-593: I would somehow clarify that the conclusions about the topology are from spch leaves, which do not have stomata.

-It might be interesting to also cite the new paper by Le Gloanec et al 2022 in Development.

-Some typos were detected, eg.:

Fig. 1A -> the ML1 abbreviation in the panel should be ATML1 for consistency.

358 typo GMX2.0 -> MGX2.0

Recommendation: Using quantitative methods to understand leaf epidermal development — R1/PR9

Comments

Comments to Author: The revision was nearly sufficient. Some more minor changes were suggested by a reviewer. Please go through them and consider if these changes would further improve the manuscript.

Decision: Using quantitative methods to understand leaf epidermal development — R1/PR10

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Author comment: Using quantitative methods to understand leaf epidermal development — R2/PR11

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Recommendation: Using quantitative methods to understand leaf epidermal development — R2/PR12

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Comments to Author: Thank you for submitting the revised manuscript.

I am pleased to say, it is now accepted for publication - congratulations!

Decision: Using quantitative methods to understand leaf epidermal development — R2/PR13

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