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Rearing and 60Co radiation do not affect attractiveness but alter the volatile profiles released by Anastrepha obliqua calling males

Published online by Cambridge University Press:  15 February 2024

Frida P. Santiago
Affiliation:
Grupo de Ecología Química, Departamento de Ecología de Artrópodos y Manejo de Plagas, El Colegio de la Frontera Sur (ECOSUR), Carretera Antiguo Aeropuerto Km. 2.5, Tapachula, Chiapas 30700, Mexico
David Alavez-Rosas
Affiliation:
Instituto de Ecología, Universidad Nacional Autónoma de México, Ciudad Universitaria, Coyoacán, CDMX 04510, Mexico
Julio C. Rojas*
Affiliation:
Grupo de Ecología Química, Departamento de Ecología de Artrópodos y Manejo de Plagas, El Colegio de la Frontera Sur (ECOSUR), Carretera Antiguo Aeropuerto Km. 2.5, Tapachula, Chiapas 30700, Mexico
*
Corresponding author: Julio C. Rojas; Email: jrojas@ecosur.mx
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Abstract

Calling males of Anastrepha obliqua release volatile compounds to attract conspecific males to form leks and females to mate. Male volatiles from Mexican and Brazilian populations of A. obliqua have been previously identified. However, there are differences in the number and identity of volatile compounds between the populations. These differences in volatile profiles may be due to male origin (e.g. wild or mass-reared flies) or methodological issues (e.g. sampling techniques). In this study, we evaluated the attractiveness of wild, laboratory non-irradiated, and laboratory-irradiated flies under semi-field conditions. Male volatiles were collected using dynamic headspace sampling (DHS) and solid-phase microextraction (SPME) techniques, and identified using gas chromatography-coupled mass spectrometry. The results showed no difference in the attractiveness of wild, laboratory non-irradiated, and irradiated males to females. However, the number of captured females differed according to the origin; wild and non-irradiated females were captured more frequently than the irradiated flies. A total of 21 compounds were found using SPME, whereas only 12 were collected using DHS, although the relative amounts of these compounds were higher than those obtained using the former sampling technique. In addition, only laboratory non-irradiated males released α-pinene and menthol, which have not been previously reported in this fruit fly species. Additionally, we identified novel compounds in A. obliqua; however, certain compounds previously reported were not detected. This study suggests that despite the qualitative and quantitative variations in the volatile profiles of A. obliqua males, their attractiveness was unaffected.

Type
Research Paper
Copyright
Copyright © The Author(s), 2024. Published by Cambridge University Press

Introduction

Male Anastrepha fruit flies (Diptera: Tephritidae) release volatile compounds during calling to attract conspecific males to form leks, and females to mate (Aluja et al., Reference Aluja, Piñero, Jácome, Diaz-Fleischer, Sivinski, Aluja and Norrbom2000). Leks take place mainly on host trees bearing fruits, where two–ten males aggregate, perch, and signal from the undersurface of leaves (Shelly, Reference Shelly2018). The pheromone seems to attract females close to the calling males but not to point sources, and at a close range, females may use acoustic and visual signals to locate males (Tan et al., Reference Tan, Nishida, Jang, Shelly, Todd, Espky, Jang, Reyes-Flores and Vargas2014).

Male volatile compounds have been identified in certain Anastrepha spp., particularly those of economic importance such as Anastrepha suspensa, Anastrepha ludens, Anastrepha obliqua, Anastrepha serpentina, and Anastrepha fraterculus (Tan et al., Reference Tan, Nishida, Jang, Shelly, Todd, Espky, Jang, Reyes-Flores and Vargas2014; Scolari et al., Reference Scolari, Valerio, Benelli, Papadopoulos and Vaníčková2021). For instance, A. obliqua males release esters, terpenes, and alcohols during calling (López-Guillén et al., Reference López-Guillén, Cruz-López, Malo and Rojas2011; Gonçalves et al., Reference Gonçalves, Silva, Mendonça, Vaníčková, Tomčala and Do Nascimento2013; Aluja et al., Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020; De Aquino et al., Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021). Nevertheless, the qualitative volatile profiles of A. obliqua varied among studies. López-Guillén et al. (Reference López-Ley, Toledo, Malo, Gómez, Santiesteban and Rojas2011) identified nine volatiles in the effluvia of mass-reared non-irradiated calling males. The major compounds identified were (Z,E)-α-farnesene, (E,E)-α-farnesene, and (Z)-3-nonen-1-ol. Later, Aluja et al. (Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020) reported up to eight compounds in wild A. obliqua males reared in hog plums (Spondias spp.), mangoes, guava, and tomatoes. Only four compounds were released by males reared in Spondias mombin, the ancestral host of A. obliqua, whereas eight compounds were found in the effluvia of males reared in guava, an occasional host of this fruit fly species. They did not find (Z)-3-nonen-1-ol in the male effluvia; instead the major compounds identified by Aluja et al. were α-bergamotene, (E,E)-α-farnesene, and (Z,Z)-3,6-nonadien-1-ol (Aluja et al., Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020). Calling A. obliqua males from Brazil reared in mangoes and carambolas released 16 and 21 compounds, respectively (Gonçalves et al., Reference Gonçalves, Silva, Mendonça, Vaníčková, Tomčala and Do Nascimento2013; De Aquino et al., Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021). The major compounds identified in later studies were 1-heptanol and ethylhexanoate. The differences found among these studies may be due to the geographical origin, host plant, or adsorbents used for sampling the volatiles. All studies collected male A. obliqua volatiles using the dynamic headspace sampling (DHS) technique with Super Q® (López-Guillén et al., Reference López-Guillén, Cruz-López, Malo and Rojas2011; Aluja et al., Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020) or Tenax® (Gonçalves et al., Reference Gonçalves, Silva, Mendonça, Vaníčková, Tomčala and Do Nascimento2013; De Aquino et al., Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021) as adsorbents. Adsorbents differ in their affinity and efficiency for trapping certain groups of compounds; therefore, an inadequate selection of the absorbent can result in ample undersampling or even deficiency to collect some volatile compounds (Noushini et al., Reference Noushini, Park, Jamie, Jamie and Taylor2020). For instance, with the solid-phase microextraction (SPME) technique, the detection limit and number of identified compounds depend on the amount and adsorbent type that coated the fibre used for sampling volatile compounds (Pawliszyn, Reference Pawliszyn1997).

In this study, we compared the attractiveness of laboratory-reared (hereafter non-irradiated and irradiated) and wild A. obliqua males to conspecific females in field cages. Subsequently, volatiles released by the three types of males were collected using DHS and static SPME techniques. Due to the differences in the reported volatiles from A. obliqua, we decided to collect volatiles with two different adsorbents for dynamic aeration and six different SPME fibres. Compounds from the extracts and fibres were identified using gas chromatography coupled with mass spectrometry (GC-MS). We hypothesised that rearing and radiation would affect male attractiveness and the profile of volatiles released during calling activity.

Materials and methods

Insects

Non-irradiated and irradiated A. obliqua pupae were provided by the MOSCAFRUT production plant (SADER-IICA) located in Metapa de Domínguez, Chiapas. The flies were reared as previously described (Artiaga-López et al., Reference Artiaga-López, Hernández, Dominguez-Gordillo, Moreno, Orozco-Dávila and Barnes2004). Sterile flies were irradiated with 60Co at 80 Gy as pupae 2 days before adult emergence. Pupae were placed in glass cages (35 cm × 35 cm × 35 cm) for adult emergence. Mango (Mangifera indica) fruits infested with A. obliqua larvae were collected from trees surrounding Tapachula, Chiapas, Mexico to obtain wild flies. Fruits were placed in plastic trays (60 cm × 52 cm × 11 cm) and covered with cloth to allow aeration. After 5–10 days, pupae were collected and placed in glass cages with vermiculite until adult emergence. Upon emergence, the flies were sexed and placed separately in cages (12 cm × 25 cm × 12 cm). Flies were fed with a mixture of sugar and hydrolysed protein (3:1), and water in a plastic container with a slightly moistened cotton swab. The flies were maintained under an artificial photoperiod of 12 h light/12 h dark at 25 ± 2°C and 70 ± 10% relative humidity. Wild flies were 12–17 days old, whereas laboratory-reared flies were 8–15 days old when used in the experiments. This difference in age is because laboratory-reared flies reach sexual maturity earlier than wild flies do (Meza-Hernández et al., Reference Meza-Hernández, Hernández, Salvador-Figueroa, Cruz-López and Barnes2002).

Male attractiveness trial

The attractiveness of A. obliqua males to conspecific females was evaluated using multiple choice tests in cylindrical nylon screen field cages (2.80 m diameter × 2.20 m high). The trials were performed under semi-natural conditions in a shaded area planted with local trees located 5 km outside of Tapachula city, Chiapas, Mexico. Ten males of a given group (i.e. wild, non-irradiated, or irradiated flies) were placed in a container of a multilure trap (Better World Manufacturing, CA, USA), which was lined with mesh to prevent the escape of males. Three traps containing live males from the three treatments were fixed at equal distances in a random manner and hung 10 cm away from the cage roof. A solution of 250 ml propylene glycol (Agrotec, Mexico) and water (1:4) was added to each trap to retain the attracted female flies. Propylene glycol does not affect the behaviour of A. obliqua (López-Ley et al., Reference López-Ley, Toledo, Malo, Gómez, Santiesteban and Rojas2016). Twenty wild, non-irradiated, and irradiated females (n = 60) were released at 08:00 h into each cage. Females from each treatment group were marked with edible dyes (Bakersfield, Chocolatera de Nayarit, Mexico). The edible dye, one colour for each fly type, was added to the water (150 μl/250 ml of water) consumed by the flies. Coloured water was supplied to flies after emergence. Thus, the abdomen of the flies was fully coloured, which made it possible to distinguish which group they belonged to when the flies were recovered from the traps. The edible dye did not affect the behaviour or survival of flies (Santiago, unpublished observations). The number of trapped flies were recorded 24 h after release, and uncaptured females were taken out from the cages and never used again. After each replication, the traps were rotated counterclockwise to minimise positional bias. In total, 32 replicates were performed.

Volatile sampling

Volatiles from the calling males were collected using DHS and static SPME. For DHS, 20 males from a given group were enclosed in a glass aeration chamber (10 cm long × 8 cm i.d.) 1 h before they began to call. Volatiles were drawn from the aeration chamber using air, previously passed through an activated carbon filter, into a collection trap. Air was drawn through a collection trap at a rate of 2.0 litres min−1. The volatile collection trap contained 50 mg of ORBO Tenax® TA (a porous polymer based on 2,6-diphenyl-p-phenylene oxide, 35–60 mesh, 100/50 mg; Merck, Darmstadt, Germany) or Super Q® (a copolymer made of ethylvinylbenzene-divinylbenzene, Porapak Q®, 50–80 mesh, 100/50 mg; Merck, Darmstadt, Germany). Male volatiles were collected during peak calling (07:00–11:00 h) at 25 ± 2°C, 60–80% relative humidity, and 557 lx illumination. The volatiles were eluted from the adsorbent with 1 ml of hexane (high-performance liquid chromatography-grade) and the extracts were concentrated to 100 μl using a gentle N2 airstream. The extracts were stored in glass vials (1 ml) at −20°C until analysis. Ten replicates were performed for each type of adsorbent.

For the SPME sampling, we used six different fibres: bare fused silica (FS), 50/30 μm divinylbenzene/carboxen/polydimethylsiloxane (DVB/CAR/PDMS), 85 μm carboxen/polydimethylsiloxane (CAR/PDMS), 75 μm carboxen/polydimethylsiloxane (CAR/PDMS), 85 μm polyacrylate (PA), and 65 μm polydimethylsiloxane/divinylbenzene (PDMS/DVB). SPME fibres were obtained from SUPELCO (Deisenhofen, Germany). Fifteen calling males were gently introduced into a 200 ml borosilicate glass Erlenmeyer flask at 09:00 h and the mouth of the flask was covered with aluminium foil and sealed with masking tape. An SPME fibre was then inserted into the flask through aluminium foil and exposed to headspace volatiles. After 30 min, the fibre was withdrawn and inserted into the GC-MS injector. An identical volatile extraction chamber was simultaneously used at the same time to determine the chemical background (emitted by the chamber or in the surrounding air). The flask with flies was maintained at 25 ± 2°C, 60–80% relative humidity, and 227 lx illumination. We used the same SPME fibre for each replicate, with a total of five replicates for each fibre type.

Chemical analysis

To identify the compounds, SPME samples and extracts from the DHS technique were analysed using a GC-MS Shimadzu GC-2010 plus Triple-Quadrupole TQ8040 (Texas, USA). A DB-5MS non-polar capillary column (30 m × 0.25 mm I.D., Supelco, Bellafont, PA) was used. The injector was operated in split mode. Helium was used as a carrier gas at 1.0 ml min−1. The oven temperature was programmed at 50°C for 2 min, followed by a ramp of 15°C for 1 min until 280°C, and held for 10 min. Ionisation was caused by the electron impact at 70 eV. The compounds were identified using the Kovats retention indices and mass spectra that matched the NIST library. Comparisons with the pure standards were performed when available.

Statistical analysis

Analyses were performed using the statistical software R version 4.3.0 (R Core Team, 2023). A general linear model with Poisson distribution was performed using Tukey's test (α < 0.05) (De Mendiburu and Simon, Reference De Mendiburu and Simon2015) to test for differences in capture between the males used in traps and the females used as responders. Insect capture was the response variable, whereas trap (male type) and female type were the response factors. The relative amounts of volatile compounds released by males were compared individually among the adsorbents using a one-way analysis of variance. Data were checked for normal distribution using the Kolmogorov–Smirnov test and for homoscedasticity with the Levene test. A heatmap was generated to compare the relative amounts of captured compounds among the different adsorbents.

Results

Male attractiveness

No differences were observed in the number of A. obliqua females captured, regardless of the origin of the males placed inside the traps (X 2 = 1.99, df = 2, P = 0.37). However, the number of females attracted by males differed depending on their origin (X 2 = 12.21, df = 2, P < 0.01). It was observed that irradiated females were less attracted to the traps than were non-irradiated and wild females (fig. 1).

Figure 1. Female capture (mean ± SE) in the semi-field bioassay: (a) female type in traps and (b) male type in traps. Different letters indicate the differences among treatments according to the Tukey's test (α = 0.05).

Sampling analysis

Twenty-five compounds were collected from the headspace of A. obliqua calling males. Qualitative differences were observed between the static and dynamic techniques used. The static technique captured up to 21 compounds, while the dynamic technique detected 12 compounds (fig. 2). Additionally, semi-quantitative differences among the adsorbents used were observed in the relative amounts of the compounds (fig. 3).

Figure 2. Chromatograms from the A. obliqua headspace and from two different adsorbents were selected. SPME (PDMS/DVB fibre) from static collection and Super Q from dynamic collection. Compounds 3 (carbitol) and 7 (phenyl ethyl alcohol) were only observed using other SPME fibre types.

Figure 3. Heatmap representing chemical analysis of volatile compounds emitted by A. obliqua males. Compounds were identified by GC-MS. The scale of the heat map represents the relative amounts (percentages) of the compound abundance. The first letter of the acronyms corresponds to male type (I: irradiated, F: fertile, and W: wild), while the second and third letters correspond to the adsorbent used (S: Super Q, T: Tenax, and the following for the SPME fibres: bare FS, 50/30 μm divinylbenzene/carboxen/polydimethylsiloxane (DCP), 85 μm carboxen/polydimethylsiloxane (85CP), 75 μm carboxen/polydimethylsiloxane (CP), 85 μm PA, and 65 μm polydimethylsiloxane/divinylbenzene (PD).

Dynamic headspace

Twelve compounds were collected from male A. obliqua using Super Q (Supp. table S1). The major compounds identified were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol (these two compounds co-elute), (E,Z)-3,6-octadien-1-ol, and cis-muurola-3,5-diene (fig. 3). α-Pinene was detected only in non-irradiated males. The relative amounts of seven compounds varied among the three groups. Wild males released higher relative amounts of 2-ethyl-1-hexanol, tetradecane, and (Z,E)-α-farnesene than non-irradiated and irradiated males. Wild and irradiated males emitted more relative amount of cis-muurola-3,5-diene, trans-calamenene, unidentified terpene, and farnesene epoxide than non-irradiated males. In contrast, there were no differences in the relative amounts of (E,Z)-3,6-octadien-1-ol, (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol, ϒ-elemene, and (E,E)-α-farnesene among wild, non-irradiated, and irradiated males.

Twelve compounds were adsorbed by Tenax (Supp. table S2), similar to those collected by Super Q. The major compounds were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol and (E,Z)-3,6-octadien-1-ol (fig. 3). The compound α-pinene was found only in the bouquet of non-irradiated males. The relative amounts of four compounds varied among the three male groups. Wild males emitted higher amounts of n-tetradecane, an unidentified terpene, than non-irradiated and irradiated males. Wild and non-irradiated males released more 2-ethyl-1-hexanol than irradiated males, whereas non-irradiated and irradiated males emitted more (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol than wild males. In contrast, no differences were observed for (E,Z)-3,6-octadien-1-ol, cis-muurola-3,5-diene, ϒ-elemene, (Z,E)-α-farnesene, (E,E)-α-farnesene, trans-calamenene, and farnesene epoxide.

Solid-phase microextraction

Twenty-one compounds were captured by the coated 65 μm PDMS/DVB fibres (Supp. table S3). The major compounds were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol and (Z,E)-α-farnesene (fig. 3). The only qualitative difference was observed for α-pinene, which was only produced by non-irradiated males. Our results showed significant differences in the relative amounts of most volatile compounds released by the different male groups. However, only there were differences among the three groups with phenol and 1-undecene. Overall, there were no significant differences in the relative amounts of these compounds between non-irradiated and irradiated males.

Twenty-one volatile compounds were collected from the coated 75 μm CAR/PDMS fibres (Supp. table S4). The major compounds in the three male groups were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol (fig. 3). The compounds α-pinene, 1-undecene, 2-ethyl-1-hexanol, and menthol were recovered only from the volatiles of non-irradiated males. Phenol, (E,Z)-3, 6-octadien-1-ol, α-guaiene, ϒ-amorphene, unidentified terpenes 1, 2, and 3, and farnesene epoxide were not found in the effluvia of wild males. In contrast, the last group of males produced more (Z,E)-α-farnesene, (E,E)-α-farnesene, and β-elemenone than irradiated and non-irradiated males. The relative amount of n-tetradecane was higher in irradiated males than in non-irradiated and wild males, whereas non-irradiated males released a higher amount of n-tetradecane than wild males. The relative amounts of β-elemene and caryophyllene were higher in irradiated and wild males than in non-irradiated males. In contrast, the relative amounts of (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol, bergamotene, and ϒ-elemene were not significantly different among the three types of males.

Twenty-one compounds were collected from the coated FS fibres (Supp. table S5). The major compounds in the three male groups were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol, (Z,E)-α-farnesene, and β-elemenone (fig. 3). The compounds α-pinene and menthol were only found in the volatiles of non-irradiated males. Phenol, (E,Z)-3,6-octadien-1-ol, 1-undecene, 2-ethyl-1-hexanol, α-guaiene, ϒ-amorphene, unidentified terpenes 1, 2, and 3, and farnesene epoxide were not recovered from the effluvia of wild males. The relative amounts of (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol, n-tetradecane, β-elemene, caryophyllene, bergamotene, ϒ-elemene, (Z,E)-α-farnesene, (E,E)-α-farnesene, and β-elemenone did not vary among the male groups.

Twenty-one compounds were collected using the coated 50/30 μm DVB/CAR/PDMS fibres (Supp. table S6). The major compounds in the three male groups were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol, (Z,E)-α-farnesene, and β-elemenone (fig. 3). The compounds α-pinene, phenol, and menthol were recovered only from the volatiles of non-irradiated males. (E,Z)-3,6-Octadien-1-ol, 1-undecene, α-guaiene, ϒ-amorphene, unidentified terpenes 1, 2, and 3, and farnesene epoxide were not found in the volatiles of wild males. Higher relative amounts of 2-ethyl-1-hexanol, β-elemene, and ϒ-elemene were found in the effluvia of wild males than in those of non-irradiated and irradiated males. The relative amount of caryophyllene was higher in the effluvia of wild and irradiated males than in that of non-irradiated males. In contrast, the relative amounts of (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol, n-tetradecane, bergamotene, (Z,E)-α-farnesene, (E,E)-α-farnesene, and β-elemenone were similar among the male groups.

Twelve compounds were collected using the coated 85 μm CAR/PDMS fibres (Supp. table S7). The major compounds in the three male groups were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol and (E,E)-α-farnesene (fig. 3). Phenol, (E,Z)-3,6-octadien-1-ol, 2-ethyl-1-hexanol, unidentified terpene 3, and farnesene epoxide were not found in the effluvia of wild males. In contrast, caryophyllene and β-elemenone were only detected in the volatiles of wild males, whereas α-guaiene was only recovered from non-irradiated males. Wild and non-irradiated males produced more (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol than irradiated males, whereas the opposite was true for n-tetradecene. No differences were observed in the relative amounts of β-elemene, (E,E)-α-farnesene, or farnesene epoxide among the male groups.

Ten compounds were collected from the coated 85 μm PA fibres (Supp. table S8). The major compounds in the three male groups were (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol (fig. 3). Phenol, carbitol, (E,Z)-3,6-octadien-1-ol, phenylethyl alcohol, ϒ-amorphene, and unidentified terpene 3 were not recovered from the effluvia of wild males. β-Elemenone was only found in the volatiles of wild males. Irradiated and non-irradiated males released more (E,Z)-3,6-nonadien-1-ol/3-nonen-1-ol than wild-type males, whereas the opposite was true for (E,E)-α-farnesene and α-guaiene.

Discussion

In the present study, we found that wild, non-irradiated, and irradiated A. obliqua males were equally attractive to the conspecific females. Our results also showed that the number and relative amounts of volatile compounds released by calling males were influenced by male source and sampling method. Despite the variation in volatile profiles, male attractiveness was not affected, suggesting that rearing and radiation did not influence the synthesis of behaviour-relevant compounds. Thus, the data obtained partially supports our working hypothesis. In addition, we identified several novel compounds in A. obliqua; however, we were unable to find some of the previously reported compounds.

Several studies have reported that radiation and artificial rearing can affect the sexual competitiveness of Anastrepha males compared with their wild counterparts (Meza-Hernández et al., Reference Meza-Hernández, Hernández, Salvador-Figueroa, Cruz-López and Barnes2002; Rull et al., Reference Rull, Brunel and Mendez2005; Gallardo-Ortiz et al., Reference Gallardo-Ortiz, Pérez-Staples, Liedo and Toledo2018). For instance, Meza-Hernández et al. (Reference Meza-Hernández, Hernández, Salvador-Figueroa, Cruz-López and Barnes2002) found that mass-reared A. obliqua males competed with wild males for wild females. However, wild females prefer wild males to mass-reared ones. The last authors also reported that mass-reared males emitted less pheromone than their wild counterparts. They speculated that this is a disadvantage for mass-reared males, as female attraction depends on the amount of male pheromone. However, our data showed that the attractiveness of laboratory-reared (non-irradiated and irradiated) and wild A. obliqua males to conspecific females was similar. Hence, our data do not align with the findings of Meza et al. (Reference Meza-Hernández, Hernández, Salvador-Figueroa, Cruz-López and Barnes2002). Thus, our results showed that at a distance, females could not discriminate among the volatiles of the different types of males. This suggests that discrimination is likely performed within a close range using acoustic, visual, or chemical signals. Anastrepha males produce two sounds in sexual context: calling sound and precopulatory sound (Sivinski et al., Reference Sivinski, Burk and Webb1984; Briceño et al., Reference Briceño, Hernández, Orozco and Hanson2009). When electing potential partners, Anastrepha females reject conspecific smaller males, which generate calling songs with a higher fundamental frequency and longer intervals between bursts (Mankin et al., Reference Mankin, Malavasi, Aquino, McPheron and Steck1996). The acoustic songs of A. suspensa males are affected by radiation from cesium-137 (Webb et al., Reference Webb, Sivinski and Smittle1987). To the best of our knowledge, the influence of rearing and radiation on the acoustic songs of A. obliqua males has not been investigated.

There were differences in the number of volatile compounds captured using the SPME and DHS techniques. Volatile compounds released by A. obliqua males into the atmosphere are perceived by females at a distance from their release point, thus mediating sexual behaviour. The identity and relative amounts (ratio or proportion) of such compounds convey specific information about the physiological state of males (Meza-Hernández et al., Reference Meza-Hernández, Hernández, Salvador-Figueroa, Cruz-López and Barnes2002). Thus, it is important to perform a robust chemical analysis of these compounds to reduce biases when interpreting their behavioural importance (Noushini et al., Reference Noushini, Park, Jamie, Jamie and Taylor2020). For this purpose, both dynamic and static samplings were used. Using SPME, 21 volatile compounds were collected from wild, non-irradiated, and irradiated male A. obliqua. The higher sensitivity of this technique allows the collection of more compounds in shorter periods of time. However, this technique has some limitations, mostly in terms of the quantitation of compounds (Cagliero et al., Reference Cagliero, Mastellone, Marengo, Bicchi, Sgorbini and Rubiolo2021). In terms of sensitivity, the coated 65 μm PDMS/DVB fibre was the most effective for collecting volatiles from A. obliqua males. Twelve volatile compounds were collected by DHS. It is possible that this technique collected fewer compounds because it requires an extended sampling time to collect sufficient volatiles (Alborn et al., Reference Alborn, Bruton and Beck2021). However, A. obliqua males exhibit calling behaviour for a few hours. Additionally, we observed that A. obliqua males were under stress during dynamic volatile collection because of the noise caused by the pumps or airflow in the pull system. This stress could affect calling behaviour and the release of compounds. Despite its low sensitivity, it is possible to perform quantitative analysis of the compounds. Both adsorbents used in this study were suitable for sampling volatiles from male A. obliqua.

Both methods used to sample the headspace of A. obliqua males have advantages and disadvantages that are strongly related to the physical and chemical properties of the adsorbent, concentration of the released volatiles, chemical properties of the compounds, and diffusion of the volatiles in the collection chamber (Angelopoulos and Pickett, Reference Angelopoulos and Pickett1998; Noushini et al., Reference Noushini, Park, Jamie, Jamie and Taylor2020; Alborn et al., Reference Alborn, Bruton and Beck2021). Ten compounds were collected in common using both sampling methods. The compounds cis-muurola-3,5-diene and trans-calamene were only captured by DHS, whereas menthol was only adsorbed by the SPME fibres. In this context, Super Q®, Tenax®, and the 65 μm PDMS/DVB fibre were the most suitable options for capturing volatiles from A. obliqua males.

Most of the compounds identified in this study have not been identified previously. For instance, we identified (E,Z)-3,6-octadien-1-ol, a possible precursor or decomposition product of (E,Z)-3,6-nonadien-1-ol, in the three types of flies, whereas α-pinene was only found in non-irradiated males. We identified eight compounds that were previously found in the effluent of A. obliqua males. For example, males of A. obliqua from Veracruz, Mexico reared on mangoes, as in our case, released only three compounds in common with A. obliqua males from Chiapas, Mexico: 3,6-nonadien-1-ol, (Z,E)-α-farnesene, and (E,E)-α-farnesene. It is possible that (Z)-3-nonen-1-ol is released by A. obliqua males from Veracruz, but the authors have not been able to identify it because it co-elutes with 3,6-nonadien-1-ol. The compounds 3,6-nonadien-1-ol, (Z,E)-α-farnesene, and (E,E)-α-farnesene are also emitted by A. obliqua males from Veracruz reared on Spondias spp., guava, and Solanum lycopersicum, a non-natural host of A. obliqua (Aluja et al., Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020). Males of A. obliqua from Brazil and Chiapas reared in mangoes released six common compounds: 3,6-nonadien-1-ol, (Z,E)-α-farnesene, (E,E)-α-farnesene, 2-ethylhexane-1-ol, β-elemene, and caryophyllene (Gonçalves et al., Reference Gonçalves, Silva, Mendonça, Vaníčková, Tomčala and Do Nascimento2013).

We do not know the possible functions of most of the compounds identified in this study in the physiology and ecology of A. obliqua. Only two studies have evaluated some of the compounds released by A. obliqua males (López-Guillén et al., Reference López-Guillén, Cruz-López, Malo and Rojas2011; De Aquino et al., Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021). In semi-field tests, López-Guillén et al. (Reference López-Guillén, Cruz-López, Malo and Rojas2011) found that more females and males were captured by traps baited with (Z)-3-nonen-1-ol and (Z,E)-α-farnesene than unbaited traps. Unfortunately, the responses of flies to these compounds were not compared with those of live calling males or calling male extracts to determine whether these compounds explain the attraction of flies to calling males or whether it is necessary to add other compounds. Later, De Aquino et al. (Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021) reported that 1-heptanol, linalool, (Z)-3-nonen-1-ol, (Z,E)-α-farnesene, and (E,Z)-3,6-nonadien-1-ol released by A. obliqua males from Brazil elicited antennal responses from conspecific females. A quaternary blend composed of the first four compounds attracted more females than male calling extracts in laboratory assays. Interestingly, 1-heptanol and linalool were not emitted by A. obliqua males in Mexico (López-Guillén et al., Reference López-Guillén, Cruz-López, Malo and Rojas2011; Aluja et al., Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020; this study). This suggests that there is geographic variation in the chemical communication of A. obliqua. Previous studies have reported that A. obliqua from Mexico mate in the morning, whereas A. obliqua from Brazil mate in the afternoon (Aluja et al., Reference Aluja, Jácome, Birke, Lozada and Quintero1993; Henning and Matioli, Reference Henning and Matioli2006). Further studies are required to confirm whether there is variation in the chemical communication of this fruit fly species.

Some of the compounds (e.g. α-pinene, caryophyllene, β-elemene, α-guaiene, bergamotene) identified in the effluvia of A. obliqua calling males have also been reported in mangoes and other natural hosts of this fruit fly species. At first glance, one might believe that these compounds are contaminants. However, the fact that these compounds were found in the volatiles of mass-reared males that did not have contact with mangoes seems to rule out this possibility. Previous studies on Anastrepha fruit flies have reported that some male compounds are emitted by their host plants. De Aquino et al. (Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021) found compounds such as 1-heptanol, limonene, linalool, and ethyl octanoate in the effluvia of A. obliqua calling males, which also have been identified in fruits of mangoes and Spondias spp. (Pino et al., Reference Pino, Mesa, Muñoz, Martí and Marbot2005; de Sousa Galvão et al., Reference de Sousa Galvão, Narain, dos Santos and Nunes2011). The pheromone of Anastrepha striata is composed of ethyl hexanoate, linalool, and ethyl octanoate (Cruz-López et al., Reference Cruz-López, Malo and Rojas2015), which are constituents of the host fruit volatiles of Anastrepha spp. (Pino et al., Reference Pino, Mesa, Muñoz, Martí and Marbot2005; de Sousa Galvão et al., Reference de Sousa Galvão, Narain, dos Santos and Nunes2011). Diaz-Santiz et al. (Reference Diaz-Santiz, Rojas, Cruz-López, Hernández and Malo2016) reported that both female and male A. striata were attracted to a six-component blend isolated from guava consisting of ethyl butyrate, (Z)-3-hexen-1-ol, hexanol, ethyl hexanoate, hexyl acetate, and ethyl octanoate. The fact that male pheromones and fruit volatiles of Anastrepha spp. share some common attractive compounds suggests that they can use the same sensory mechanisms in both sexual and host plant locations.

One of the limitations of our study is that most compounds were identified using Kovats retention indices and mass spectra that matched the NIST library. Unfortunately, in many cases, these compounds are not commercially available, and their synthesis is complicated. Future studies should confirm the identification of these compounds, particularly those ecologically relevant to A. obliqua. For example, Aluja et al. (Reference Aluja, Cabagne, Altúzar-Molina, Pascacio-Villafán, Enciso and Guillén2020) identified (Z,Z)-3,6-nonadien-1-ol in the effluvia of A. obliqua males. However, it was not possible to discern between the (Z,Z) and (E,Z) isomers using GC-MS. The retention indices of both isomers are almost the same: 1156 and 1161, respectively. Because we had a retention index of 1161, we were inclined to believe that the isomer was (E,Z), coupled with the fact that De Aquino et al. (Reference De Aquino, Ferreira, Tavares, Silva, Mendonça, Joachim-Bravo, Milet-Pinheiro, Navarro, De Abreu Galdino and Do Nascimento2021) reported that this isomer is bioactive. Further studies (e.g. nuclear magnetic resonance analysis) are needed to determine whether the isomer is (E,Z) or (Z,Z).

In summary, we did not find any differences in the attractiveness of wild, sterile, and fertile A. obliqua males. In addition, a robust chemical analysis of volatiles from males revealed differences in the chemical profiles of the different types of males. We identified volatile compounds released by A. obliqua calling males that have not been reported in previous studies with this species. Further studies are needed to investigate the role of the identified compounds in the behavioural ecology of A. obliqua. Ecologically relevant compounds can be used for the monitoring or mass trapping of this fruit fly species.

Supplementary material

The supplementary material for this article can be found at https://doi.org/10.1017/S000748532400004X.

Acknowledgements

We thank Azucena Oropeza, Johana Gonzalez, and Fernando Cortes (ECOSUR) for their help in collecting infested mangoes and technical support, and the Moscafrut (National Fruit Fly Campaing-SADER-IICA) mass-rearing facility for providing mass-reared flies. This study was funded by the International Agency of Atomic Energy (grant no. 24796). F. P. S. acknowledges ECOSUR for a scholarship.

Competing interests

None.

Ethical approval

Not applicable: the study did not include mammalian subjects.

References

Alborn, HT, Bruton, RG and Beck, JJ (2021) Sampling of volatiles in closed systems: a controlled comparison of three solventless volatile collection methods. Journal of Chemical Ecology 47, 930940.CrossRefGoogle ScholarPubMed
Aluja, M, Jácome, I, Birke, A, Lozada, N and Quintero, G (1993) Basic patterns of behavior in wild Anastrepha striata (Diptera: Tephritidae) flies under field-cage conditions. Annals of the Entomological Society of America 86, 776793.CrossRefGoogle Scholar
Aluja, M, Piñero, J, Jácome, I, Diaz-Fleischer, F and Sivinski, J (2000) Behavior of flies in the genus Anastrepha (Trypetinae: Toxotrypanini). In Aluja, M and Norrbom, AL (eds), Fruit Flies (Tephritidae): Phylogeny and Evolution of Behavior. Boca Raton, USA: CRC Press, pp. 375406.Google Scholar
Aluja, M, Cabagne, G, Altúzar-Molina, A, Pascacio-Villafán, C, Enciso, E and Guillén, L (2020) Host plant and antibiotic effects on scent bouquet composition of Anastrepha ludens and Anastrepha obliqua calling males, two polyphagous tephritid pests. Insects 11, 309. https://doi.org/10.3390/insects11050309CrossRefGoogle ScholarPubMed
Angelopoulos, NG and Pickett, JA (1998) Headspace analysis in chemical ecology: effects of different sampling methods on ratios of volatile compounds present in headspace samples. Journal of Chemical Ecology 24, 11611172.CrossRefGoogle Scholar
Artiaga-López, T, Hernández, E, Dominguez-Gordillo, J, Moreno, DS and Orozco-Dávila, D (2004) Mass-production of Anastrepha obliqua at the moscafrut fruit fly facility, Mexico. In Barnes, BN (ed.), Proceedings of the 6th International Symposium on Fruit Flies of Economic Importance. Irene, South Africa: Isteg Scientific Publications, pp. 389392.Google Scholar
Briceño, RD, Hernández, M, Orozco, D and Hanson, P (2009) Acoustic courtship songs in males of the fruit fly Anastrepha ludens (Diptera: Tephritidae) associated with geography, mass rearing and courtship success. Revista de Biología Tropical 57, 257265.Google Scholar
Cagliero, C, Mastellone, G, Marengo, A, Bicchi, C, Sgorbini, B and Rubiolo, P (2021) Analytical strategies for in-vivo evaluation of plant volatile emissions – a review. Analytica Chimica Acta 1147, 240258.CrossRefGoogle ScholarPubMed
Cruz-López, L, Malo, EA and Rojas, JC (2015) Sex pheromone of Anastrepha striata. Journal of Chemical Ecology 41, 458464.CrossRefGoogle ScholarPubMed
De Aquino, NC, Ferreira, LL, Tavares, R, Silva, CS, Mendonça, A, Joachim-Bravo, IS, Milet-Pinheiro, P, Navarro, D, De Abreu Galdino, FC and Do Nascimento, RR (2021) Bioactive male-produced volatiles from Anastrepha obliqua and their role in attraction of conspecific females. Journal of Chemical Ecology 47, 167174.CrossRefGoogle ScholarPubMed
De Mendiburu, F and Simon, R (2015) Agricolae – ten years of an open source statistical tool for experiments in breeding, agriculture and biology. PeerJ PrePrints 3, e1404v1. https://doi.org/10.7287/peerj.preprints.1404v1Google Scholar
de Sousa Galvão, M, Narain, N, dos Santos, MDSP and Nunes, ML (2011) Volatile compounds and descriptive odor attributes in umbu (Spondias tuberosa) fruits during maturation. Food Research International 44, 19191926.CrossRefGoogle Scholar
Diaz-Santiz, E, Rojas, JC, Cruz-López, L, Hernández, E and Malo, EA (2016) Olfactory response of Anastrepha striata (Diptera: Tephritidae) to guava and sweet orange volatiles. Insect Science 23, 720727.CrossRefGoogle ScholarPubMed
Gallardo-Ortiz, U, Pérez-Staples, D, Liedo, P and Toledo, J (2018) Sexual competitiveness, field survival, and dispersal of Anastrepha obliqua (Diptera: Tephritidae) fruit flies irradiated at different doses. Journal of Economic Entomology 111, 761769.CrossRefGoogle ScholarPubMed
Gonçalves, GB, Silva, CE, Mendonça, ADL, Vaníčková, L, Tomčala, A and Do Nascimento, RR (2013) Pheromone communication in Anastrepha obliqua (Diptera: Tephritidae): a comparison of the volatiles and salivary gland extracts of two wild populations. Florida Entomologist 96, 13651374.CrossRefGoogle Scholar
Henning, F and Matioli, SR (2006) Mating time of the West Indian fruit fly Anastrepha obliqua (Macquart) (Diptera: Tephritidae) under laboratory conditions. Neotropical Entomology 35, 145148.CrossRefGoogle ScholarPubMed
López-Guillén, G, Cruz-López, L, Malo, EA and Rojas, JC (2011) Olfactory responses of Anastrepha obliqua (Diptera: Tephritidae) to volatiles emitted by calling males. Florida Entomologist 94, 874881.CrossRefGoogle Scholar
López-Ley, JU, Toledo, J, Malo, EA, Gómez, J, Santiesteban, A and Rojas, JC (2016) Carambola cultivar, fruit ripeness, and damage by conspecific larvae influence the host-related behaviors of Anastrepha obliqua (Diptera: Tephritidae). Journal of Economic Entomology 109, 154160.CrossRefGoogle Scholar
Mankin, RW, Malavasi, A and Aquino, C (1996) Acoustical comparisons of calling songs from Anastrepha species in Brazil. In McPheron, BA and Steck, GJ (eds), Fruit Fly Pests. Boca Raton, USA: CRC Press, pp. 3742.Google Scholar
Meza-Hernández, JS, Hernández, E, Salvador-Figueroa, M and Cruz-López, L (2002) Sexual compatibility, mating performance and sex pheromone release of mass-reared and wild Anastrepha obliqua (Diptera: Tephritidae) under field-cage conditions. In Barnes, BN (ed.), Proceedings of the 6th International Symposium on Fruit Flies of Economic Importance. Irene, South Africa: Isteg Scientific Publications, pp. 99104.Google Scholar
Noushini, S, Park, SJ, Jamie, I, Jamie, J and Taylor, P (2020) Sampling technique biases in the analysis of fruit fly volatiles: a case study of Queensland fruit fly. Scientific Reports 10, 19799.CrossRefGoogle ScholarPubMed
Pawliszyn, J (1997) Solid Phase Microextraction: Theory and Practice. New York, USA: John Wiley & Sons, 264p.Google Scholar
Pino, JA, Mesa, J, Muñoz, Y, Martí, MP and Marbot, R (2005) Volatile components from mango (Mangifera indica L.) cultivars. Journal of Agricultural and Food Chemistry 53, 22132223.CrossRefGoogle ScholarPubMed
R Core Team (2023) R: A Language and Environment for Statistical Computing. Vienna, Austria: R Foundation for Statistical Computing. https://www.R-project.org/Google Scholar
Rull, J, Brunel, O and Mendez, M E (2005) Mass rearing history negatively affects mating success of male Anastrepha ludens (Diptera: Tephritidae) reared for sterile insect technique programs. Journal of Economic Entomology 98, 15101516.CrossRefGoogle ScholarPubMed
Scolari, F, Valerio, F, Benelli, G, Papadopoulos, NT and Vaníčková, L (2021) Tephritid fruit fly semiochemicals: current knowledge and future perspectives. Insects 12, 408.CrossRefGoogle ScholarPubMed
Shelly, TE (2018) Sexual selection on leks: a fruit fly primer. Journal of Insect Science 18, 9, 1–16.CrossRefGoogle ScholarPubMed
Sivinski, J, Burk, T and Webb, JC (1984) Acoustic courtship signals in the Caribbean fruit fly, Anastrepha suspensa (Loew). Animal Behaviour 32, 10111016.CrossRefGoogle Scholar
Tan, KH, Nishida, R, Jang, EB and Shelly, TE (2014) Pheromones, male lures, and trapping of tephritid fruit flies. In Todd, S, Espky, N, Jang, EB, Reyes-Flores, J and Vargas, R (eds), Trapping and the Detection, Control, and Regulation of Tephritid Fruit Flies: Lures, Area-Wide Programs, and Trade Implications. Dordrecht, The Netherlands: Springer, pp. 1574.CrossRefGoogle Scholar
Webb, JC, Sivinski, J and Smittle, BJ (1987) Acoustical courtship signals and sexual success in irradiated Caribbean fruit flies (Anastrepha suspensa) (Diptera: Tephritidae). Florida Entomologist 70, 103109.CrossRefGoogle Scholar
Figure 0

Figure 1. Female capture (mean ± SE) in the semi-field bioassay: (a) female type in traps and (b) male type in traps. Different letters indicate the differences among treatments according to the Tukey's test (α = 0.05).

Figure 1

Figure 2. Chromatograms from the A. obliqua headspace and from two different adsorbents were selected. SPME (PDMS/DVB fibre) from static collection and Super Q from dynamic collection. Compounds 3 (carbitol) and 7 (phenyl ethyl alcohol) were only observed using other SPME fibre types.

Figure 2

Figure 3. Heatmap representing chemical analysis of volatile compounds emitted by A. obliqua males. Compounds were identified by GC-MS. The scale of the heat map represents the relative amounts (percentages) of the compound abundance. The first letter of the acronyms corresponds to male type (I: irradiated, F: fertile, and W: wild), while the second and third letters correspond to the adsorbent used (S: Super Q, T: Tenax, and the following for the SPME fibres: bare FS, 50/30 μm divinylbenzene/carboxen/polydimethylsiloxane (DCP), 85 μm carboxen/polydimethylsiloxane (85CP), 75 μm carboxen/polydimethylsiloxane (CP), 85 μm PA, and 65 μm polydimethylsiloxane/divinylbenzene (PD).

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