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Skin Models Used to Define Mechanisms of Action of Sulfur Mustard

Published online by Cambridge University Press:  18 October 2023

Jeffrey D. Laskin*
Affiliation:
Department of Environmental and Occupational Health and Justice, Rutgers University School of Public Health, Piscataway, NJ, USA
Kevin Ozkuyumcu
Affiliation:
Department of Pharmacology and Toxicology, Ernest Mario School of Pharmacy, Piscataway, NJ, USA
Peihong Zhou
Affiliation:
Department of Pharmacology and Toxicology, Ernest Mario School of Pharmacy, Piscataway, NJ, USA
Claire R. Croutch
Affiliation:
MRIGlobal, Kansas City, MO, USA
Diane E. Heck
Affiliation:
Department of Pharmacology and Toxicology, Ernest Mario School of Pharmacy, Piscataway, NJ, USA
Debra L. Laskin
Affiliation:
Department of Pharmacology and Toxicology, Ernest Mario School of Pharmacy, Piscataway, NJ, USA
Laurie B. Joseph
Affiliation:
Department of Pharmacology and Toxicology, Ernest Mario School of Pharmacy, Piscataway, NJ, USA
*
Corresponding author: Jeffrey D. Laskin PhD; Email: jlaskin@eohsi.rutgers.edu.
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Abstract

Sulfur mustard (SM) is a threat to both civilian and military populations. Human skin is highly sensitive to SM, causing delayed erythema, edema, and inflammatory cell infiltration, followed by the appearance of large fluid-filled blisters. Skin wound repair is prolonged following blistering, which can result in impaired barrier function. Key to understanding the action of SM in the skin is the development of animal models that have a pathophysiology comparable to humans such that quantitative assessments of therapeutic drugs efficacy can be assessed. Two animal models, hairless guinea pigs and swine, are preferred to evaluate dermal products because their skin is morphologically similar to human skin. In these animal models, SM induces degradation of epidermal and dermal tissues but does not induce overt blistering, only microblistering. Mechanisms of wound healing are distinct in these animal models. Whereas a guinea pig heals by contraction, swine skin, like humans, heals by re-epithelialization. Mice, rats, and rabbits are also used for SM mechanistic studies. However, healing is also mediated by contraction; moreover, only microblistering is observed. Improvements in animal models are essential for the development of therapeutics to mitigate toxicity resulting from dermal exposure to SM.

Type
Systematic 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 (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution and reproduction, provided the original article is properly cited.
Copyright
© The Author(s), 2023. Published by Cambridge University Press on behalf of Society for Disaster Medicine and Public Health, Inc

Sulfur mustard (SM, bis 2-chloroethyl sulfide) is a potent skin vesicant synthesized for chemical warfare. As a bifunctional alkylating agent, SM initiates its action by modifying and disrupting cellular macromolecules, including DNA and proteins. Reference Balali-Mood and Hefazi1Reference Dacre and Goldman5 Acute responses of skin to SM are typically characterized by delayed onset erythema and intense itching, followed by the formation of small fluid-filled vesicles; with time, these vesicles coalesce to form pendulous blisters. Reference Balali-Mood and Hefazi1,Reference Kehe and Balszuweit6,Reference Graham and Schoneboom7 A necrotic layer and ulceration can form on the affected skin surface following rupture of the blisters. Responses of human skin to SM are multifactorial and depend on the dose and time following exposure, as well as environmental conditions such as temperature and humidity. Reference Graham and Schoneboom7,Reference Sollman8 Location of exposure sites on the body, variations in skin properties, and underlying disease states, along with age and sex, are all determinants of skin responses to SM. Reference Sollman8

To understand the mechanism of action of SM and develop medical countermeasure, various animal models have been utilized, including mice, rats, guinea pigs, rabbits, and pigs. Reference Renshaw9Reference Young, Fabio and Huang12 Unfortunately, there are no simple or common animal models for SM injury that produce true blisters like humans. In this context, in describing early reporting on the use of human subjects for mustard research in 1919, Sollman explained that “experiments on animals was [sic] abandoned after a few trials, since their skin does not react in the same manner as human skin, and the effects that do occur are not easily graded.” Reference Sollman8 Blistering is not commonly observed in animals. Reference Rice, Brown and Lam13,Reference Flesch, Goldstone and Weidman14 To produce true blistering, either unconventional species must be used, or multistep procedures must be undertaken in common animal models. Reference Flesch, Goldstone and Weidman14 For example, it has been reported that blisters can be produced on the skin of frogs, birds, and the inner ears of rabbits, Reference Mershon, Mitcheltree and Petrali15 on the skin of isolated perfused pig flaps, Reference Mershon, Mitcheltree and Petrali15,Reference King and Monteiro-Riviere16 and on guinea pig skin that has been thermally burned and allowed to re-epithelialize. Reference King and Monteiro-Riviere16,Reference Braue, Nails and Way17 Studies performed with SM on birds and frogs are limiting as their skin is not similar to human skin. For this reason, SM research has relied on the surrogate marker of microblistering or subepidermal blister formation at the dermal-epidermal junction, which occurs in rodents, rabbits, and pigs. Reference Smith, Casillas and Graham18Reference Braue and Nalls20 SM is known to damage not only epidermal structures, including the basement membrane, but also stromal and vascular components of the skin tissue. Reference Smith, Skelton and Hobson21Reference Joseph, Composto and Heck23

Translating SM data from animals to humans has been challenging not only because there is little or no blistering, but also to additional factors such as distinct structural differences in the tissue, unique aspects of the immune system, and mechanisms of wound healing. For example, in mice, the skin and epidermis are thinner when compared to humans, there are fewer epidermal cell layers, a lack of epidermal ridges and eccrine sweat glands, and limited adherence to underlying tissues. Reference Grambow, Sorg and Sorg24 In humans and pigs, wounds close by formation of granulation tissue followed by re-epithelialization Reference Grambow, Sorg and Sorg24 ; in contrast, wound closure in rodents and rabbits is primarily by contraction, in part due to the presence of the panniculus carnosus. Reference Naldaiz-Gastesi, Bahri and Lopez de Munain25 At later stages, tissue remodeling during wound healing occurs via fibroblast migration and myofibroblast activity. Reference Tottoli, Dorati and Genta26 It should be noted that contraction is usually defined for incisional wounds Reference Masson-Meyers, Andrade and Caetano27 ; the role of contraction in thermal and SM injury is not clear since the extent of tissue damage may not allow wound closure by the panniculus carnosus.

In rodent models, both haired and hairless strains have been used; hairless animals are advantageous largely due to the ease of visualizing a cutaneous response. Reference Wormser, Brodsky and Sintov28 Hair removal and associated inflammation are avoided with these animals. Reference Braue, Nails and Way29 However, it should be noted that the skin of haired and hairless animal strains can be morphologically different. For example, the epidermis of mice of the most commonly used hairless strain, SKH1, is thicker than haired strains. Reference Renshaw9 Haired and hairless strains are also genetically and immunologically distinct, complicating efforts to compare results from different laboratories. Reference Jung and Maibach30 Little information is available on differences in wound healing in response to chemical and thermal injury in haired and hairless mouse strains.

In most animal models, different phases of SM injury can be defined, including latency, erythema/inflammation, microblistering, ulceration/eschar formation, and wound healing. The extent of injury depends on several factors, including the model, location and area of skin exposed to SM, as well as SM dose and methods of administration and environmental conditions when applying SM. Targeting one or more phases of injury is essential in the development of effective countermeasures to mitigate SM toxicity. Both clinical signs and morphological/biochemical parameters have been used to characterize the action of SM in animal models. Clinical signs are evident by visual inspection; at early times, this includes erythema, edema and transepidermal water loss (TEWL), and, at later times, extent of injury and whether injury is superficial, intermediate in depth, or deep dermal injury. Reference Braue, Nails and Way29 The integrity of the dermal-epidermal junction, measured by dermal torque, has been demonstrated in SM-treated guinea pigs. Reference Snider, Matthews and Braue31 Laser Doppler imaging has also been used to assess cutaneous blood flow and ballistometry to evaluate mechanical properties of the skin, including rigidity and elasticity in pig models. Reference Reid, Neimuth and Shumaker32,Reference Graham, Stevenson and Mitcheltree33

Techniques in histology, electron microscopy, and immunohistochemistry have been used to analyze structural alterations in skin exposed to SM. These studies have largely focused on the epidermis, basement membrane, and accessary structures, including hair follicles and sebaceous glands. Early effects of SM in basal cells of the epidermis, as reported in guinea pig skin include nuclear condensation and mitochondrial swelling, disorganization of desmosomes and hemidesmosomes, and widening of intracellular spaces in the basal cell layer. Reference Vogt, Dannenberg and Schofield19 At later times, nuclear pyknosis, cell fragmentation, and necrosis extending into suprabasal cells are evident. Reference Kan, Pleva and Hamilton34 Markers of DNA damage and apoptosis and necrosis also appear in epidermal cells. Reference Lakshmana Rao, Vijayaraghavan and Bhaskar35 Mediators of inflammation, including prostaglandins and cytokines, are also expressed after SM-induced injury. Reference Dachir, Fishbeine and Meshulam11,Reference Dachir, Cohen and Kamus-Elimeleh22 Microvesicles appear in the lamina lucida of the basement membrane as a consequence of degeneration of the basal layer. Reference Monteiro-Riviere, Inman and Babin36,Reference Petrali and Oglesby-Megee37 Proteolysis of basement membrane components, including laminins, collagens, and other anchoring proteins by matrix metalloproteinases, contributes to the disruption of the basal cell layer, microvesication, and ulceration. Reference Mouret, Wartell and Batal38,Reference Chang, Wang and Chang39 At later times, in minipig skin, aberrant epidermal proliferation and differentiation are associated with re-epithelialization including hyperplasia, hyperkeratosis, and parakeratosis. This is thought to contribute to prolonged wound healing. Reference Laskin, Wahler and Croutch40,Reference Stricker-Krongrad, Shoemake and Bouchard41

The dermis and hypodermis are also targets for SM. This is important as the integrity of these tissues is critical for wound healing. Reference Dachir, Cohen and Kamus-Elimeleh22,Reference Joseph, Composto and Heck23,Reference Reid, Graham and Niemuth42,Reference Chauhan, Murtthy and Arora43 Leukocyte infiltration, a marker of inflammation, has been observed in the dermis post-SM exposure in all animals studied. Reference Vogt, Dannenberg and Schofield19,Reference Dannenberg, Pula and Liu44Reference Tanaka, Dannenberg and Higuchi46 In mouse and guinea pig skin, mast cell degranulation is also evident, along with alterations in collagen deposition. Reference Mouret, Wartell and Batal38,Reference Graham, Bryant and Brave47,Reference Joseph, Composto and Perez48 In pig skin, SM also disrupts the dermal vasculature and subsequent blood flow, and responses can affect tissue oxygenation, possibly leading to reperfusion injury. Reference Graham, Schomacker and Glatter49,Reference Hall, Lydon and Dalton50 These pathologic responses can impair wound healing, lead to infection, and initiate scarring.

Guinea Pig Skin Model of SM Toxicity

Both haired and hairless guinea pigs have been used to assess SM toxicity with generally similar results (Table 1). Hairless guinea pigs have been reported to be more sensitive to SM in terms of the extent of dermal injury. Reference Marlow, Mershon and Mitcheltree51 These animals are also more sensitive to SM-induced epidermal necrosis compared to other animal models, including the weanling pig, mouse ear, and hairless mice. Reference Smith, Casillas and Graham18 The hairless guinea pig skin is considered morphologically more like human skin, Reference Snider, Matthews and Braue31,Reference Smith, Graham and Moeller52 which has prompted greater use of these animals to understand the mechanism of action of SM and for the development of countermeasures. Reference Barillo, Croutch and Reid53

Table 1. Effects of sulfur mustard on guinea pig skin

As indicated above, a characteristic early response of guinea pig skin to SM is a marked inflammatory response, notably, infiltration of neutrophils and macrophages into the tissue. Reference Mishra, Rir-sima-ah and March54 Mustards cause the release of inflammatory mediators, including reactive oxygen and reactive nitrogen species, and cytokines such as TNFα and IL-1α, which activate macrophages contributing to tissue injury. Reference Laskin, Black and Jan2,Reference Pohanka, Stetina and Svobodova55 This is followed by the appearance of anti-inflammatory/wound repair macrophages. Reference Biyashev, Onay and Dala56 That macrophages can contribute to wound repair is evidenced by findings that intradermal injection of activated human macrophages into SM-treated guinea pig skin can significantly improve clinical signs of tissue damage. Reference Dachir, Cohen and Sahar57

Of interest are studies by Graham et al. Reference Graham, Bryant and Brave47 showing that SM reduces mast cell numbers in hairless guinea pig skin, suggesting that degranulation may be an early marker of toxicity. These investigators hypothesized that histamine and other mediators released by mast cells may play a role in SM-induced injury. These data are in accord with studies by ours and other laboratories demonstrating mast cell degranulation and reduced number of mast cells in SM-exposed hairless mouse skin. Reference Mouret, Wartell and Batal38,Reference Joseph, Composto and Perez48 The use of antihistamine promethazine, in combination with the PARP inhibitor niacinamide, and the non-steroidal anti-inflammatory agent indomethacin in guinea pig skin, decreases mast cell degranulation. Reference Yourick, Dawson and Mitcheltree58Reference Yourick, Dawson and Benton60

Rat, Mouse, and Rabbit Models of SM Toxicity

In these models, exposure to SM is either by direct application of liquid to the skin or as a vapor (Tables 25). Vapor exposures are typically preferred since vapor is the more likely route of exposure during a mass causality scenario. Depending on the dose and environmental conditions, generally similar characteristic responses are observed following treatment of the dorsal skin of rats, mice, and rabbits with SM. Initially, there is a latency period, which is followed by a cutaneous inflammatory response characterized by erythema, edema, and leukocyte infiltration. Subsequently, there is microblister formation, tissue granulation, epidermal necrosis, and, finally, wound repair and tissue remodeling. Reference Mershon, Mitcheltree and Petrali15,Reference Chang, Soriano and Hahn61,Reference Petrali, Oglesby and Hamilton62 More detailed information has been reported on the effects of SM on hair follicles and sebaceous glands in the mouse model. Reference Joseph, Composto and Heck23,Reference Joseph, Gerecke and Heck63 In hair follicles, SM induces epithelial cell karyolysis within the hair root sheath, infundibulum, and isthmus and reduces the numbers of sebocytes in sebaceous glands. Reference Joseph, Heck and Cervelli64 Significant DNA damage and apoptosis are evident around pilosebaceous units with increased numbers of inflammatory cells surrounding utriculi. These findings may explain, at least in part, depletion of hair follicles in human skin following exposure to SM.

Table 2. Effects of sulfur mustard on rat skin

Table 3. Effects of sulfur mustard on mouse skin

Table 4. Effects of sulfur mustard in the mouse ear vesicant model

Table 5. Effects of sulfur mustard on rabbit skin

An important method that can partially overcome wound contraction and the need for fur removal is the use of the mouse ear vesicant model (see Table 4). This method is largely based on early studies showing that biological and biochemical processes associated with inflammation can easily be measured following exposure to cutaneous irritants or allergens. Reference Monteiro-Riviere, Inman and Babin36,Reference Casillas, Mitcheltree and Stemler65Reference Patrick, Burkhalter and Maibach67 In this model, SM is applied to the inner surface of the mouse ear, which is largely free of hair. Ear cartilage appears to prevent wound contraction. Reference Rajnoch, Ferguson and Metcalfe68 After a latency period, edema, measured by changes in ear weight, epidermal necrosis, and epidermal-dermal separation are assessed. Reference Casillas, Mitcheltree and Stemler65,Reference Casillas, Kiser and Truxall69 Transmission electron microscopy and immunohistochemistry have been used to identify biomarkers of injury, as well as mechanisms of subepidermal blister formation. Reference Monteiro-Riviere, Inman and Babin36,Reference Sabourin, Petrali and Casillas70

In rabbits, dorsal and ventral skin and ear skin have been used to investigate SM injury and the formation of microblisters. Reference Zlotogorski, Goldenhersh and Shafran71Reference Sun, Sun and Zheng75 In each exposure scenario, SM damage has been assessed visually by monitoring erythema, wound healing, and histopathology. Reference Vogt, Dannenberg and Schofield19,Reference Liu, Wannemacher and Snider73,Reference Sun, Sun and Zheng75,Reference Schoene, Bruckert and Schreiber76 In the rabbit models, depending on the dose, SM damages the superficial microvasculature as measured by Evans blue dye extravasation and leakage of erythrocytes. Reference Vogt, Dannenberg and Schofield19,Reference Dachir, Cohen and Fishbeine77 SM also damages fibroblasts, possibly disrupting the extracellular matrix. In contrast to the dorsal and ventral skin, rabbit ears have no panniculus carnosus; thus, wound contraction does not contribute to the healing process. Reference Nabai and Ghahary78 This model is thought to better reflect wound healing in humans. However, in a continuous flow vapor exposure model, rabbit ears have been reported to be significantly less sensitive than human skin to SM injury. Reference Schoene, Bruckert and Schreiber76

Pig Models of SM Toxicity

Pig skin is the most anatomically and physiologically similar to human skin, compared to rodents and rabbits, making it a preferable model for translational research (Tables 6 and 7). From a regulatory standpoint, considerable background data are available on pig skin related to the development of dermatological products, making this model ideal for SM countermeasure research. Pig skin is tightly attached to the subcutaneous connective tissue, contains a relatively thick epidermis, distinct rete ridges and, like human skin, dense elastic fibers in the dermis. Reference Summerfield, Meurens and Ricklin79Reference Rittie81 Pig skin hair is coarser than human hair but has a similar distribution. Reference Stricker-Krongrad, Shoemake and Bouchard41,Reference Summerfield, Meurens and Ricklin79,Reference Khiao In, Richardson and Loewa82 Although humans have eccrine glands distributed throughout their skin, swine eccrine glands are primarily found in the snout, lips, and carpal organ. Reference Seaton, Hocking and Gibran80 In the skin of both pigs and humans, re-epithelialization during wound healing is associated with basal cell proliferation and differentiation into enucleated granular cells that migrate outward toward the surface of the skin. Reference Takeo, Lee and Ito83 However, as with other animal models, SM is unable to form true blisters, a characteristic sign of toxicity in humans following vesicant exposure. Reference Kehe and Balszuweit6,Reference Graham and Schoneboom7,Reference Kehe, Thiermann and Balszuweit84

Table 6. Effects of sulfur mustard on pig skin

Table 7. Effects of sulfur mustard on pig skin

Both dorsal and ventral skin models have been used to assess SM toxicity in pig skin (see Tables 6 and 7). In general, the ventral skin of pigs is thinner and more responsive to SM than dorsal skin. Reference Pramudita, Shimizu and Tanabe85 The choice of dorsal versus ventral pig skin models is dependent on the type of exposure (eg, liquid vs vapor cap) and the type of injury being investigated (eg, superficial vs intermediate or deep dermal). Both models can be used to assess pharmaceutical preparations. However, dorsal skin is preferable with the use of wound dressings that must be maintained for prolonged periods of time (see further below). Both clinical and histopathological endpoints are used to assess tissue damage. Clinical changes include blood flow, elasticity, skin color, thickness, and spectral properties. Reference Graham, Schomacker and Glatter49,Reference Hall, Lydon and Dalton50 Histopathological changes include skin structure, epithelial and basement membrane integrity, and expression of markers of proliferation and differentiation of keratinocytes during wound healing. Reference Laskin, Wahler and Croutch40,Reference Sabourin, Danne and Buxton86Reference Chilcott, Dalton and Ashley88 Following these endpoints over time will provide information on the wound healing process and the effectiveness of potential countermeasures. Decontaminants, protectants, anti-inflammatory agents, and wound dressing have been evaluated for their ability to mitigate tissue damage induced by SM, often with varying degrees of success. Reference Plahovinsak, Buccullato and Reid89

Based on pig skin models that have been developed to assess medical countermeasures against SM-induced skin injury, one product, Silverlon® Wound Contact, Burn Contact Dressings, has been approved by the FDA. 90 Manufactured as a non-adherent knitted nylon fiber wound dressing coated with metallic silver, Silverlon® is approved for use with decontaminated, unroofed first and second degree burns induced by SM. Silverlon® also acts as an oxygen-permeable sterile barrier, which promotes wound healing. Reference Barillo, Croutch and Reid53 Silver ions in the product also serve as an antimicrobial, reducing infections at the wound site. Reference Barillo, Pozza and Margaret-Brandt91

Support for Silverlon® in the FDA approval process was based on a pathophysiological scale in the Göttingen minipig vapor cap model (Table 8). Individual endpoints indicate the extent and type of repair and include the appearance of epithelial cells, basement membrane damage, re-epithelialization of the wound, whether abnormal hair follicles are present, extent of dermal inflammation and the presence of rete ridges, vascular proliferation, and hemorrhage. Reference Graham, Stevenson and Mitcheltree33,Reference Barillo, Croutch and Barillo92 In the case of Silverlon®, approvals were based on re-epithelialization of the skin and improved appearance of the basement membrane, as well as a reduction in dermal inflammation. Silverlon® has also been FDA approved for radiation dermatitis and cutaneous radiation injury through dry desquamation. 93

Table 8. Skin histopathology scoring for evaluating sulfur mustard countermeasures using Göttingen minipigsa

Summary

Animal models are essential not only for understanding the mechanism of action of SM, but also to develop effective therapeutics. Importantly, therapeutics may be effective at different stages of SM injury (eg, during the latency prior to a cutaneous response, during the inflammatory response, or during wound healing/tissue remodeling) and can be used alone or in combination. For example, Silverlon® is effective for wound healing following the appearance of first- and second-degree burns after exposure to SM. It remains to be determined whether treatments with anti-inflammatory agents prior to the development of SM burns will improve Silverlon®-induced wound healing. Thus far, research in the field is limited as SM is a blistering agent, and none of the animal models form overt blisters in response to this vesicant. Further studies are required to better understand differences between human and animal responses to SM so that more effective countermeasures can be developed that not only enhance wound healing, but also mitigate the blistering response.

Author contributions

Jeffrey D. Laskin: conceptualization, funding acquisition, literature search, original manuscript draft writing, review & editing; Kevin Ozkuyumcu: literature search & manuscript draft writing; Peihong Zhou: manuscript review & editing; Claire R. Croutch: manuscript review & editing; Diane E. Heck: manuscript review & editing; Debra L. Laskin: funding acquisition, manuscript review & editing; Laurie B. Joseph: literature search, original manuscript draft writing, review & editing.

Funding statement

This work was supported by the National Institutes of Health Grants U54AR055073, R01ES004738, R01ES033698, and P30ES005022

Conflict(s) of interest

The authors declare no conflicts of interest.

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Figure 0

Table 1. Effects of sulfur mustard on guinea pig skin

Figure 1

Table 2. Effects of sulfur mustard on rat skin

Figure 2

Table 3. Effects of sulfur mustard on mouse skin

Figure 3

Table 4. Effects of sulfur mustard in the mouse ear vesicant model

Figure 4

Table 5. Effects of sulfur mustard on rabbit skin

Figure 5

Table 6. Effects of sulfur mustard on pig skin

Figure 6

Table 7. Effects of sulfur mustard on pig skin

Figure 7

Table 8. Skin histopathology scoring for evaluating sulfur mustard countermeasures using Göttingen minipigsa