Drosophila melanogaster chemical ecology revisited: 2-D distribution maps of sex pheromones on whole virgin and mated flies by mass spectrometry imaging

Background

Sexual behavior in Drosophila melanogaster flies is greatly influenced by chemical cues. In this study, a spatial distribution of female and male sex pheromones was investigated on the surface of virgin and mated six-day-old fruit flies. Surface analysis was performed using the technique of mass spectrometry imaging (MSI) matrix-assisted laser desorption/ionization – time of flight (MALDI-TOF) and confirmed by gas chromatography – mass spectrometry (GC-MS) analysis of hexane extracts prepared from dissected flies.

Results

MALDI-TOF MSI experiments focused on female pheromones (7Z,11Z)-heptacosa-7,11-diene (7,11-HD) and (7Z,11Z)-nonacosa-7,11-diene (7,11-ND) were enhanced by using lithium 2,5-dihydroxybenzoate (LiDHB) matrix to improve the ionization and quality of MS spectra. Oxygenated compounds represented by male anti-attractants 11-cis-vaccenyl acetate (cVA) and 3-O-acetyl-1,3-dihydroxy-octacosa-11,19-diene (CH503) were successfully ionized without MALDI matrix in the form of potassium adducts in laser desorption ionization (LDI-TOF MSI) mode. A similar pattern of distribution for 7,11-HD and 7,11-ND was observed on the surface of both the left and the right female wing, with the strongest signals at the base of the wing. 7,11-HD and 7,11-ND were additionally detected on female legs but not on the body. The distribution of both male pheromones, cVA and CH503, was localized in virgin male flies solely on the abdominal tip and anogenital region. In addition, results from MSI experiments with mated flies showed the distribution of cVA and CH503 also on the female abdomen and thorax, demonstrating that anti-attractants were transferred from males to females during copulation. Results from LDI/MALDI-TOF MSI were supported by GC-MS analysis of hexane extracts prepared from different parts of virgin male or female Drosophila flies. Similar amounts of 7,11-HD and 7,11-ND were present on the legs, body and wings (127 ± 5 ng and 170 ± 8 ng, respectively). cVA was detected only on the male body. All acquired MSI datasets were affected by mass shift (predominantly between ±0.2 Da to ±0.4 Da), which was reduced using a mass recalibration approach.

Conclusions

The LDI/MALDI-TOF MSI technique makes it possible to study the distribution of female and male sexual pheromones on D. melanogaster flies. Moreover, the technique enables the transfer of male sex pheromones to females during copulation to be visualized. However, imaging experiments of 3-D biological samples performed on a single TOF-MS instrument equipped with a MALDI ion source and UV nitrogen laser evinced a photo-electric charging/discharging, a phenomenon that often leads to unpredictable mass shifts and poor mass accuracy.

Sexual behavior in Drosophila melanogaster flies is influenced by non-chemical and chemical cues. Non-chemical signals include visual and acoustic stimuli; for example, male flies visually track the movement of females [1, 2] and produce a courtship song by vibrating one or both wings to initiate mating [3,4,5]. However sounds can also be emitted in the same way by females in order to attract males [6]. Although the auditory component of the wing-vibration song has been thoroughly investigated [7], whether wing vibration is also involved in the dispersal of pheromones is unknown.

Chemical cues in Drosophila include sex pheromone signals. Volatile pheromones in Drosophila [8,9,10] as well as close-range sex pheromones in D. melanogaster are well known, including hydrocarbons and oxygenated hydrocarbons that can be perceived either by olfactory organs, such as antennae or maxillary palps; by contact with the tarsae; or by gustatory receptors on the proboscis [11, 12]. One of the best-known Drosophila sex pheromones is 11-cis-vaccenyl acetate (cVA), which plays a dual role as a short-lived inhibitor of male courtship and as an aggregation pheromone [13,14,15]. Furthermore, cVA is a male pheromone that is synthesized in the ejaculatory bulb [13] and transferred from males to females during mating [16]. The presence of cVA on a mated female has been shown to reduce its attractiveness to males for several hours [17]. Another D. melanogaster male sex pheromone, 3-O-acetyl-1,3-dihydroxy-octacosa-11,19-diene (CH503), is also an inhibitor of male courtship. Unlike cVA, CH503 remains on the female cuticle for more than 10 days [18]. In addition to male-specific pheromones, the female-specific sex pheromones (7Z,11Z)-heptacosa-7,11-diene (7,11-HD) and (7Z,11Z)-nonacosa-7,11-diene (7,11-ND) are both thought to serve as attractants for males [19].

Mass spectrometry imaging (MSI) is a method for visualizing the two-dimensional (2-D) spatial distribution of compounds of interest across a sample’s entire imaged area. MSI provides a rastering of the sample line by line and simultaneously desorbs/ionizes its surface, typically using an ultraviolet laser and MALDI technology. In order to enhance the quality of MS spectra and to ionize specific groups of compounds, a MALDI matrix is applied on the sample [20].

Compared with conventional techniques used to detect pheromones or semiochemicals, MSI provides not only a 2-D distribution of the desired compound over the entire surface of the analyzed sample but also (via MS signal intensity) its relative quantity within a lateral distribution. This information can be obtained for a hundreds of different compounds in a single MSI experiment. When MSI is applied to a Drosophila fly sample, a 2-D image can be constructed for particular m/z ratios; these ratios can represent chemical cues present on a fly cuticle [20].

In our previous studies, we have shown a presence of 7,11-HD and 7,11-ND on Drosophila melanogaster female wings [21] and the presence of cVA on males [22]. These data were acquired and used in order to demonstrate the utility of the LiDHB matrix [23] and the usefulness of a newly developed MSI data recalibration method [24]. We now hope to use these results to help address long-standing biological questions [8, 25].

Although the behavioral and physiological functions of the different pheromones are well understood, in this study, we describe their detailed 2-D distribution on the body surface of D. melanogaster and link the spatial occurrence of the pheromones with the fly’s sexual behavior. Here we discuss the pros and cons of applying the MALDI-TOF MSI method to study questions in chemical ecology.

To support our MSI data, we dissected the legs, wing and body parts of entire flies, after briefly washing them in hexane, and quantified the surface lipids via GC-MS analysis.

Insect material

D. melanogaster (Meigen, 1830) flies (Diptera, Drosophilidae) were obtained from a colony (strain Canton S) maintained at the Max Planck Institute for Chemical Ecology in Jena, Germany. We analyzed 6-day-old flies, each of which was bred separately (isolated at the pupal stage) in an Eppendorf tube (2 mL) at 25 °C, 70% humidity and a 12/12 h light darkness circle. Flies were fed for 4 days on a normal diet (30 mg of solid food - recipe shown in Table S1 – plus a moistened tissue on the bottom of the vial to prevent food from drying out) and for the last 2 days on sugar solution only to eliminate food contamination of the fly surface. To obtain mated pairs of fruit flies, a female fly and a male fly were placed in a refrigerator (4 °C) and cooled for approximately 3 min before being put together into a new Eppendorf tube. The copulation was carried out at laboratory temperature, and pairs were immobilized at − 20 °C immediately afterward. Virgin flies were immobilized the same way.

Fly samples were warmed slowly (sealed in plastic Eppendorf tubes) to room temperature prior to being fixed onto dedicated MALDI targets.

Chemicals

2,5-Dihydroxybenzoic acid (DHB) for MALDI MS with purity above 98% was purchased from Sigma-Aldrich. Lithium 2,5-Dihydroxybenzoate (LiDHB) matrix was synthesized as described previously [23]. High purity MS grade solvents (acetone, ethanol, methanol, dichloromethane) were also supplied by Sigma-Aldrich (Germany) as well as analytic-grade poly (ethylene glycol) oligomers (PEG with average masses of 200 Da, 300 Da, 600 Da and 1000 Da) for calibration of the mass spectrometer. 11-cis-vaccenyl acetate (cVA), (7Z,11Z)-heptacosa-7,11-diene (7,11-HD) and (7Z,11Z)-nonacosa-7,11-diene (7,11-ND) standards were purchased from Cayman Chemicals (Germany).

MALDI imaging

LDI/MALDI-TOF imaging experiments of D. melanogaster flies were performed on MALDI Micro MX (Waters, UK) pumped down from 1 × 10^− 6 up to 9 × 10^− 7 mbar and operated in reflectron mode with the acceleration and plate voltages at − 12 kV and 5 kV, respectively. Extraction pulse duration was set to 500 ns. Desorption and ionization were achieved using MNL 103-LD pulsed nitrogen laser (337.1 nm; pulse half width 3 ns; pulse energy ≥90 μJ; repetition rate up to 30 Hz; LTB Lasertechnik Berlin, Germany). Matrix ions were suppressed, and the low mass cut-off was set at 150 Da.

Intact flies were fixed into complex profiled cells imprinted on a dedicated aluminum MALDI plate [20] using two-part resin epoxy glue (Hardman®, www.royaladhesives.com, Belleville, NJ, USA). LiDHB matrix solution was prepared in acetone:dichloromethane (9:1, v/v) at a concentration of 20 mg/mL. The matrix was sprayed on fly samples before drying by a commercial airbrush (Harder & Steenbeck, www.airbrushuniverse.com, Norderstedt, Germany) with a 0.15 mm diameter nozzle from a distance of 160 mm. For one sample, 2 mL of LiDHB matrix solution was used to form approximately 60 layers. LiDHB matrix prepared in MeOH (20 mg/mL) was applied on fixed female wings and legs using SunChrom MALDI spotter (SunChrom GmbH, Germany) and this spraying method: line distance 2 mm, spraying speed 800 mm/min with 5 s drying time and with a flow rate of 60 μL/min. After matrix application, whole intact fly samples were placed into a desiccator with solid potassium hydroxide at ambient temperature and pressure for 6 h; dissected wings and legs, 1 h. After that time, the samples were completely dry and ready for imaging experiments.

Samples of flies were imaged using a step size of 100 μm. The number of laser shots per spot was optimized and set to 120 (60 μJ/shot) at a laser repetition rate of 15 Hz for MALDI-TOF MSI experiments (30 Hz for the samples of fly legs & wings) and 40 shots (60 μJ/shot) per spot at a laser repetition rate of 5 Hz for LDI-TOF MSI. The range of measured masses was set from 100 Da to 1000 Da and 300 Da to 550 Da for the samples of fly legs and wings, respectively. The typical laser ablation spot of 30 Hz/120 shots (60 μJ/shot) is represented by an oval area 40 μm × 60 μm from where most of the energy is focused. The outer ring is 70 μm × 90 μm.

Data were acquired with MassLynx 4.0 software and processed with custom-made software MALDI Image Convertor (Waters, UK) to obtain laterally differentiated data. These datasets were then analyzed with a method developed in-house and recalibrated in order to eliminate mass shift. Recalibrated MSI datasets were subsequently converted to 2-D ion intensity maps.

Recalibration of MSI dataset

The acquired imaging datasets affected by mass shift were imported into MATLAB (MATLAB and Statistics Toolbox Release R2012b, The MathWorks®, Inc., Natick, Massachusetts, USA) using available protocols. In order to improve the quality of the MS spectra, each dataset was subjected to the following preprocessing steps: baseline correction using the msbackadj MATLAB routine (Bioinformatics Toolbox) and smoothing using mslowess MATLAB routine (Bioinformatics Toolbox). Next, peak-picking was performed using the mspeaks routine available in MATLAB. For every dataset, the peaklists were exported as individual text files along with their coordinate position information.

Peaklists belonging to every dataset were recalibrated using the lock mass-free mass spectra recalibration approach proposed by Kulkarni et al. [24]. To rearrange the order of peaklists for recalibration, out of the two peaklist ordering approaches proposed by Kulkarni et al., the crystal growth (CG) ordering approach was applied. MSICorrect software implementing this recalibration approach can be downloaded from https://bio.informatik.uni-jena.de/software/msicorrect/.

GC-MS analysis of sex pheromones in hexane extracts of D. melanogaster

The samples were measured on an Agilent 7890A gas chromatograph (Agilent Technologies, CA) running in splitless mode and connected to an Agilent 5975C mass spectrometer (electron ionization mode, 70 eV, ion source: 230 °C, quadrupole: 150 °C, mass scan range: m/z 50–450). For GC-MS analysis, 1 μL of each sample was injected on a polar column (HP-INNOWAX, 30 m length, 0.25 mm ID, 0.25 μm film thickness, J&W Scientific) which was operated under constant helium flow (1 mL/min). The GC oven was kept at 40 °C for 1 min, ramped at 20 °C/min to 260 °C and then kept at 260 °C for 20 min.

Compounds were identified by comparing mass spectra to authentic reference compounds in our databases, based on predicted fragmentation patterns, or to those published by the National Institute of Standards and Technologies.

Sample preparation of wing hexane extracts of virgin D. melanogaster females

The hexane extracts for GC-MS analysis of male and female pheromones were prepared separately from 5 flies of each sex. For these and all other experiments, we used flies from the Canton S strain. Male and female flies were cut into three parts: wings, legs, and head/thorax/abdomen. Micro-scissors and tweezers were carefully cleaned in hexane before every cutting step, and the preparation was performed in such a way as to eliminate any cross-contamination of fly body parts. Fifteen samples obtained from 5 males and 5 females were collected in glass inserts and mixed with 60 μL of hexane. After 30 s of extraction, performed at laboratory temperature, 4 μL of internal standard n-C16 diluted in hexane at a concentration of a 50 ng/μL was added to the mixture. The supernatant was removed by glass capillary, transferred to a new glass insert and subsequently dried using a gentle stream of argon to a marked level of 20 μL. The final concentration of C16 standard for each sample was 10 ng/μL.

Sample preparation of anogenital extracts of virgin D. melanogaster males

In contrast to the sample preparation of wing extracts, the anogenital extracts of male fruit flies had to be prepared manually by rubbing specific regions of the male fly body with small pieces of paper. For each experiment, 14 male fruit flies were selected. The anogenital region of each fly was rubbed with blotting paper that had been pre-extracted with hexane and cut with scissors into small pieces (1 mm × 2 mm). Each piece of paper was soaked in hexane using tweezers and then used to gently wipe the abdominal tip and the genital area. The procedure was repeated twice with new paper for each individual fly. Obtained papers containing extracts of surface lipids were collected in glass inserts and extracted with hexane (40 μL). Individual samples were prepared as specified in the description of hexane extracts of wings.

Surface area of virgin D. melanogaster females

The surface of the whole female fly was measured using a Keyence digital microscope VHX-5000 equipped with a zoom lens VHX-J20T (Keyence Germany GmbH, Germany). Measurements were performed on several six-day-old virgin female flies with a length of 2.5 mm, representing the average size of female flies. First wings, then legs, were cut from the thorax and their dimensions measured. After that, the body of the fly was cut into head, thorax and abdomen, and measured. Obtained dimensions of each part were averaged from three individual female flies, and the surface was calculated using the formula for a cylinder or a cuboid surface area. Based on our measurements, the total surface area of one Drosophila female fly corresponded to 22.55 mm². The average surface area of female legs was approximately 2.9 mm², of wings, approximately 11.5 mm², and of the rest of the fly body surface area, ca 8.2 mm². For details, see Table S2.

Scanning electron microscopy

Images of D. melanogaster were obtained using a scanning electron microscope (SEM) Zeiss (LEO) 1450VP (Carl Zeiss AG, Germany). The scanning microscope was also used to study the quality of the LiDHB layer deposited on the flies by spraying. The MALDI targets with flies on them were coated with a thin layer (20 nm thick) of gold using SCD 050 (Bal-Tec, Liechtenstein) sputter coater. The targets were fixed by conductive carbon double-sided tape (Ted Pella Inc., USA) onto a 3-D holder in the SEM chamber. Images were made using the acceleration voltage of 10 kV.

Dedicated MALDI targets designed for previously published LDI/MALDI-TOF MSI experiments of the whole D. melanogaster flies [20] meet the requirements for experiments presented in this study, including MSI performed on flies which were imaged from ventral side.

The sex pheromones analyzed via LDI-TOF MSI mode were predominantly detected in the form of adducts with potassium and sodium ([M + K]⁺; [M + Na]⁺) cations, both of which are naturally present on the fly cuticle [21, 22, 24].

The mass spectra recalibration process applied to MSI datasets significantly reduced the mass shift [24]. In addition, the quality of MSI allowed us to generate 2-D ion intensity maps; these were improved by manual peak-picking, which was part of the recalibration method that helped to recognize and include even low-intensity MS signals.

Effect of fly handling, matrix deposition, and drying

Several experiments using an optical digital microscope and a scanning electron microscope were performed to investigate the potentially negative effects of drying on the chemical composition of the fly cuticle. We wanted to investigate what happens when the fly abdomen – lacking the mechanical support provided by our dedicated MALDI target [22] – dries out.

Based on detailed images obtained by SEM, we showed that the abdominal cuticle in particular evinces very high flexibility and compactness under the stress caused by shrinkage related to drying. We did not observe any visible damage, such as cracks or clefts, in the tergites during this process (Fig. S1).

When the quality of the LiDHB layer deposited on the fly via spraying was investigated using SEM, the images showed uniform coverage: the matrix was spread across the entire surface of the wings. Matrix deposition formed by multiple layer depositions using both a manual airbrush, and SunChrom MALDI spotter provided a uniform layer of matrix aggregated in densely packed lens-like isles with ca 30 μm diameter and a distance between of ca 50 μm (Fig. S2 a, b, c, d). As the laser ablation area is 40 μm × 60 μm and the step size 100 μm, we consider the matrix deposition to be uniform.

MALDI-TOF MSI of female pheromones on virgin D. melanogaster females

MSI experiments of virgin D. melanogaster female flies was expected to reveal the distribution of the sexual pheromones 7,11-HD and 7,11-ND. Unfortunately, ionization and visualization of these hydrocarbons was problematic. The main problem was the volatility of these dienes under vacuum pressure (up to 9.10^− 7 mbar). Notably, previously published LDI profiling data acquired under much higher pressure (2–4 mbar) [18] clearly showed adduct ions of these dienes, supporting the usefulness of pressure for detecting the pheromones under LDI conditions. Because it was not possible to work in the LDI-TOF mode, an application of LiDHB MALDI matrix on the flies was necessary to prevent pheromone loss in the vacuum by its co-crystallization with the matrix. Matrix deposition onto the fly surface also helped to increase the ionization of pheromones (Fig. S3). In order to minimize the loss of 7,11-HD and 7,11-ND from the fly cuticle, the matrix was applied on dissected female wings and legs, and intact female flies by spraying immediately after samples were fixed on the MALDI target. The samples were subsequently placed into a desiccator and allowed to dry under atmospheric pressure for 6 h in the case of whole flies and 1 h for wings or legs.

Based on the results from MALDI-TOF MSI experiments, the distribution of both female pheromones, 7,11-HD and 7,11-ND, was localized on the wings and legs of females; the strongest signals were observed at the base of the wings and on the hindmost two segments of the legs. These signals were symmetrical on both wings of single female flies and were similar among females (Fig. 1). The same distribution of 7,11-HD and 7,11-ND was obtained from the dorsal and ventral side of the wings (data not shown). The ion intensity maps (Fig. 1a, d) corresponding to the preferably formed lithium adduct of 7,11-HD at m/z 383.4 ([M + Li]⁺) and 7,11-ND at m/z 411.4 ([M + Li]⁺) suggest that both dienes were concentrated at the base of the wings.

The distribution of the female sex pheromones 7,11-HD and 7,11-ND obtained from two pairs of intact wings originating from two six-day-old virgin D. melanogaster females. The dataset was obtained by MALDI-TOF MSI in positive ion mode with LiDHB matrix applied using SunChrom MALDI spotter. (a) A 2-D ion intensity map of 7,11-HD at m/z 383.4 ([M + Li]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.4 Da. (b) The observed mass shift of m/z 383.4 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (c) The mass shift correction of m/z 383.4 signal made after applying the recalibration method. (d) A 2-D ion intensity map of 7,11-ND at m/z 411.4 ([M + Li]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.4 Da. (e) The observed mass shift of m/z 411.4 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (f) The mass shift correction of m/z 411.4 signal made after applying the recalibration method

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In MALDI-TOF MSI of female wings, we chose a mass window of ±0.4 Da to visualize the ion maps, despite the rather planar wings, because the region of the wing base was always elevated (by approximately 300 μm) compared to the rest of the sample. Due to the higher thickness of this wing area, it was the location of a mass shift.

Results from MALDI-TOF MSI of female wings were supported by a GC-MS analysis of hexane extracts of female wings; MS spectra obtained from these analyses confirmed presence of both female pheromones (Fig. S4). Yet the signals from 7,11-HD and 7,11-ND visualized in MSI experiments performed on whole intact female flies were weak (Fig. S3). Despite the fact that we almost did not see hydrocarbons in MSI of whole female flies, there were many signals corresponding to unknown signals (Fig. S5) and symmetrically distributed on the wing base.

Distribution of 7,11-HD and 7,11-ND on legs of virgin females

Although distribution of female dienes at the base of the wings was unexpected, their distribution on legs reported by Yew et al. was not [18]. We confirmed these results presented by Yew et al. by analyzing samples of dissected legs. The sample preparation protocol had to be modified to obtain sufficient signal intensity. Due to the hairy surface of the fly leg and its very small outer diameter (in a range of 25 μm to 60 μm in the case of the tarsi and tibia), epoxy glue could not be applied to the whole length. Therefore, only the femur end of the leg was fixed to the MALDI plate. Allowing leg flexibility could have resulted - in combination with an ablation plume - in slight movement during measurement. Nevertheless, realistic MSI data were obtained (Fig. 2) after mass recalibration (Fig. 2c,f), and 7,11-HD and 7,11-ND were shown to exhibit a similar lateral distribution on both tarsi and tibia, with the highest intensity for 7,11-ND.

The distribution of the female sex pheromones 7,11-HD and 7,11-ND within one set of legs originating from one six-day-old virgin D. melanogaster female. The dataset was obtained by MALDI-TOF MSI in positive ion mode with LiDHB matrix applied using SunChrom MALDI spotter. (a) A 2-D ion intensity map of 7,11-HD at m/z 383.42 ([M + Li]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±1.0 Da. (b) The observed mass shift of m/z 383.4 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (c) The mass shift correction of m/z 383.42 signal made after applying the recalibration method. (d) A 2-D ion intensity map of 7,11-ND at m/z 411.45 ([M + Li]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±1.0 Da. (e) The observed mass shift of m/z 411.45 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (f) The mass shift correction of m/z 411.45 signal made after applying the recalibration

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Legs and wings were also prepared on the normal MALDI target (Fig. S6). Reconstructed images for the lateral distribution of both 7,11-HD and 7,11-ND on wings show similar signal intensities to those on legs, with the highest signals measured on the tarsi.

MALDI spectra show a pronounced mass shift in both the blue and the red regions (see Fig. 2e). Without mass spectra recalibration [24], the signals are shifted even up to 1 Da, and signal annotation is complicated. On the other hand, laser irradiation of an individual spot results in a correct mass readout and no mass shift is observable (Fig. S7). We assume that the hairy structures (Fig. S2f) on legs accumulate an electric charge after prolonged UV-laser irradiation during MSI, and even when legs are mounted on a metallic target or on carbon tape, the charge imposed in a high vacuum barely dissipates (data not shown).

LDI-TOF MSI of male pheromones on virgin D. melanogaster males

Another set of MSI experiments focused on the male-specific sex pheromones cVA [8] and CH503 [18], and their distribution on the cuticles of virgin male flies. Measurements were carried out in LDI-TOF positive mode (without the LiDHB matrix) because the oxygenated nature of these compounds resulted in efficient ionization, unlike the unsaturated hydrocarbons represented by female pheromones. In virgin flies, both pheromones were found only in males and both were similarly distributed exclusively on the lower part of the male abdomen (Fig. 3).

The distribution of the male sex pheromones cVA and CH503 within one pair of intact six-day-old virgin D. melanogaster flies. The dataset was obtained by LDI-TOF MSI in positive ion mode. (a) A 2-D ion intensity map of cVA at m/z 349.2 ([M + K]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.4 Da. (b) The observed mass shift of cVA represented as a 2-D ion intensity map in PlusMinus 1 color scale. (c) The mass shift correction of m/z 349.2 signal made after applying recalibration method. (d) A 2-D ion intensity map of CH503 at m/z 503.3 ([M + K]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.4 Da. (e) The observed mass shift of CH503 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (f) The mass shift correction of m/z 503.3 signal made after applying the recalibration method

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Identical LDI experiments in which we fixed virgin males and females on the MALDI target on their dorsal side to visualize CH503 and cVA at the ventral anogenital region showed the presence of both pheromones only in virgin males (Fig. 4).

The distribution of male sex pheromones cVA and CH503 within one pair of intact six-day-old virgin D. melanogaster flies. The dataset was obtained by LDI-TOF MSI in positive ion mode. (a) A 2-D ion intensity map of cVA at m/z 349.6 ([M + K]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.1 Da. (b) The observed mass shift of cVA represented as a 2-D ion intensity map in PlusMinus 1 color scale. (c) The mass shift correction of m/z 349.6 signal made after applying recalibration method. (d) A 2-D ion intensity map of CH503 at m/z 503.3 ([M + K]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.4 Da. (e) The observed mass shift of CH5O3 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (f) The mass shift correction of m/z 503.3 signal made after applying the recalibration method

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Similar results confirming the presence of cVA solely in male flies were obtained by GC-MS analysis of paper material used for rubbing the anogenital region of virgin males (Fig. S8). Surprisingly, we did not identify any CH503 in our GC-MS spectra. Its relatively high molecular weight and its low thermal stability under GC conditions may have caused compound degradation.

Transfer of male-specific sex pheromones to females during copulation

We next tested whether our analysis could also be used to document the described transfer of pheromones from male to females during mating. In order to perform imaging experiments with mated males and females, one six-days-old virgin male and female fly (both reared individually) were placed into a plastic tube and kept together till the end of their copulation. The act of copulation and also the courtship were recorded on camera, and the obtained footage was studied afterwards. MSI experiments with mated flies were carried out in LDI-TOF mode. Unlike virgin females (Fig. 3a), mated females had a strong signal of cVA and CH503 on both the dorsal (Fig. 5) and the ventral (Figure S9) sides of the wing. Although the ventral signal was expected, due to its close contact with the male anogenital region during mating, the presence of cVA on the female abdomen and the male thorax (Fig. 5a) was striking.

The transfer of male sex pheromones cVA and CH503 within one pair of intact six-day-old copulated D. melanogaster flies. The dataset was obtained by LDI-TOF MSI in positive ion mode. (a) A 2-D ion intensity map of cVA at m/z 349.5 ([M + K]⁺) with signal intensity displayed in voxel view and rainbow-color coded within a mass window of ±0.2 Da. (b) The observed mass shift of cVA represented as a 2-D ion intensity map in PlusMinus 1 color scale. (c) The mass shift correction of m/z 349.5 signal made after applying the recalibration method. d) A 2-D ion intensity map of CH503 at m/z 503.8 ([M + K]⁺) with signal intensity in voxel view and rainbow-color coded within a mass window of ±0.3 Da. (e) The observed mass shift of CH503 represented as a 2-D ion intensity map in PlusMinus 1 color scale. (f) The mass shift correction of m/z 503.8 signal made after applying the recalibration method

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GC-MS analyses of female and male hexane washes

The fast hexane extraction of dissected wings, legs and the remaining body with an internal standard added to the mixture provided rich extracts from each sex; all were subsequently analyzed using GC-MS. The identity of described compounds is based on typical fragmentation patterns of EI-MS spectra, and 31 compounds were quantified in female samples (Table S3, Fig. S10). Pheromone dienes were found to occur in similar quantities in all dissected tissues. Wings and especially the body contain a level of saturated compounds that is likely related to the protection they provide against water evaporation (Fig. 6a). However, if a surface area of individual samples of wings, legs and rest of the body (Table S2) is assigned with the quantitative GC-MS data it revealed a disparity between samples. The legs with smallest area shown highest concentration of dienes per squere millimeter of sample surface (Fig. 6b) and the wings and body exhibit approximately 3 times and 2.5 times lower concentration, respectively. No trace of cVA was detected in any tissues.

An abundance of compounds is detected in hexane washes of dissected wings, legs and the remaining body parts. (a) Amounts are calculated using internal standard (b) The amounts divided by surface areas are reported in Table S2. N = 5. For compound identification, see Table S3

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To deduce the distribution of cVA from MSI data, we analyzed male extracts. As expected, cVA was present on male body parts only (Fig. S11). Other components identified included a series of saturated and 2-methyl branched saturated hydrocarbons from C21 to C31, and monoenic hydrocarbons from C21 to C29. No dienes or CH503 were detected.

Our MALDI MSI experiments revealed a distribution of female pheromones 7,11-HD and 7,11-ND on female wings, with the strongest signals at the wing base. We also observed signals from 7,11-HD and 7,11-ND in the wing blade area (Fig. 1a). This symmetrical pattern, which was found on both the dorsal and the ventral sides of the wing, might be explained by the presence of capillaries connecting pheromone gland outlets localized in the wing base region with the rest of the wing. Deployment of pheromones onto the wing blade area could lead to increases in spreading of the pheromones. In contrast to the previous explanation, which is the spread of female pheromones to the wing blade via the legs, is reflected in the symmetry of the pheromone distribution, that is, the presence of pheromones on both the dorsal and the ventral wing sides. As a similar distribution of corresponding dienes at the wing base was observed on the wings of the grayflesh fly (Neobellieria bullata) [21], we believe this distribution may be common in other Hymenoptera.

On the other hand, imaging experiments using whole Drosophila flies showed weaker signals compared to experiments using dissected wings. Because the base of the dissected wings is never directly connected to the metal MALDI target, poor contact may explain the weak signals in female HCs; electric charging, poor ion extraction and trapped ions in this region, all of which result from poor contact, are known to lower signal intensities in MS spectra [22]. In addition, the oxygenated compounds in the wing base region most likely increased after the LiDHB matrix was sprayed on the fly. (When matrix is sprayed on a fly prior to drying, the extraction of lipids -- especially from deeper cuticle layers -- is facilitated.) [24]. Therefore, the poor ion extraction in combination with preferential ionization of oxygenated compounds (presented on the surface) against hydrocarbons emerged in very low intensity of 7,11-HD and 7,11-ND ions in MS spectra.

Legs have been reported to be bearing the highest amount of dienes in Drosophila [18]. Our MSI experiments confirmed this finding: both tarsi and tibia showed high amounts of dienes. The MSI data were supported by GC-MS data from hexane extracts of dissected fly parts.

Monoenes and dienes are biosynthesized from fatty acids of different chain length by the enzyme delta-9 fatty acid desaturase [26, 27]. Formed monoenic acids are elongated/decarboxylated to odd-carbon-number monoenes in both males and females. Female flies possess the desatF desaturase working on monoenic acid providing dienic acids on carbon, which are elongated/decarboxylated to odd-carbon-number dienes [28]. The second desaturation step is under control of Antennapedia and Bithorax gene complexes, and a factor originating from prothorax has a great influence on the production of dienes in abdominal segments 4 to 5. The dienes are most likely produced in oenocytes [29]. Synthetized hydrocarbons are afterwards transported by lipophorines circulating in hemolymph. This can explain the ubiquitous occurrence of dienes in all parts of the female body. On the other hand, that male sex pheromones are mostly localized in specialized parts of the body, such as pheromonal glands, is well known from Lepidoptera. In Drosophila, female sex pheromones are recognized by specific receptors localized on male legs [30]. Dienes represent overall signal of femininity to males.

Our MSI experiments focused on male sexual pheromones showed a similar distribution of cVA and CH503 (Figs. 3 and 4). As cVA and CH503 are co-localized, they most probably occurred in a mixture. Our conclusions are supported with findings published by Yew et al. [18] showing by in situ MS profiling that cVA and CH503 are co-localized at the tip of the male fly ejaculatory bulb, in which cVA is stored [25] and in which also the last biosynthetic step of cVA takes place [31]. Accordingly, we suggest that CH503 might be also stored in the ejaculatory bulb. CH503 biosynthesis is under control of the Bond gene, which is expressed on the reproductive organ epithelium [32], and CH503 can be profiled from this area. However, based on recently published work by Niehoff et al. [33] and Khalil et al. [34], CH503 seems to be more widespread than cVA and can be detected in the entire posterior area of the male flies.

The courtship videos (Fig. 7) revealed that a male not only comes into contact with the female abdominal tip during copulation, but also probes the female with its legs (Fig. 7a) and proboscis (Fig. 7c) as described by Guiraudie-Capraz [31]. Those are the parts of the female - wings and abdomen - that according to our analysis, after courtship carries the male-specific pheromones. Additional evidence that the male could use its legs to transfer specific biologically active compounds comes from Yew et al., who documented the transfer of female pheromones to male legs after copulation [18].

Male courtship is a potential means by which pheromones are transferred. (a) The male fly taps with legs on the side of the female abdomen. (b) The male fly approaches the female from behind and taps on the upper part of the female abdomen, which is located under the wings. (c) The copulation attempt is preceded by the male tapping on the female anogenital region

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In addition, our MSI results of whole Drosophila flies also demonstrated that both male pheromones are spread over the entire male abdomen (especially on the dorsal side). Such coverage could be achieved partly by the passive diffusion of pheromones in a layer of cuticular lipids but more likely by using the hindmost pair of legs.

MALDI MSI using the LiDHB matrix exhibits a dramatic mass shift that originates from laser-induced electric charging/discharging on the surface of the flies. Using the computational recalibration approach, mass shift can be considerably reduced. Nevertheless, ionization is sometimes suppressed (as we observed on the female fly body), possibly by the presence of oxygenated compounds on the fly cuticle, likely triacylglycerols. Using LiDHB under high vacuum is the only known way to image saturated hydrocarbons, as has been shown in bees [35]. Another method for cuticle profiling, developed in Dreisewerd’s laboratory and named FALDI [36], uses UV-LDI mass spectrometry on orthogonal-flight instrument geometry; however, as yet this method is unable to ionize saturated hydrocarbons. The ion yield strongly depends on the pressure in the source, and in commercial instruments, such pressure is not easily controlled.

A dedicated aluminum MALDI target with imprinted shaped grooves for male and female flies allowed us to analyze in LDI or MALDI mode the distribution of pheromones on both the dorsal and the ventral sides of Drosophila flies. The distribution of hydrocarbons represented by female pheromones 7,11-HD and 7,11-ND was studied on virgin and mated female flies via MALDI-TOF MSI with a LiDHB matrix. Signals from the pheromones revealed a symmetrical pattern for the left and right female wings, with the strongest signals located at the base of the wings. No difference was observed between virgin and mated female flies, and no signals of 7,11-HD or 7,11-ND were observed on virgin or mated male flies. The distribution of male cVA and CH503 pheromones, also visualized in LDI-TOF MSI, on virgin males was identical. These pheromones are exclusively present on the abdominal tip and the anogenital region. The situation was slightly different in the MSI of mated females. MSI clearly indicates that both compounds are transferred simultaneously during copulation onto the female. Moreover, our experiments suggest which part of the female body males transfer their pheromones to during mating.

As the transfer of male pheromones significantly reduces female sexual attractiveness to other males [19], these imaging experiments based on 2-D visualization confirm the role of cVA and CH503 as male-transferred anti-attractants. Results from all MSI experiments were supported by GC-MS analyses of hexane extracts of specific parts of both male and female flies. GC-MS results confirmed the presence of 7,11-HD or 7,11-ND in the extracts of female wings and also that of cVA in samples prepared by rubbing the anogenital region of males and the abdominal tips of mated females. The presence of both female pheromones and cVA in the MS spectra was confirmed by analyzing standards under the same experimental conditions (Figs. S8 and S12). That CH503 was not, however, found in the GC-MS spectra - most likely it was degraded under the GC conditions - highlights the sensitivity and usefulness of MALDI-TOF.

The datasets used and/or analyzed during the current study are stored at Mass spectrometry/Proteomics Research Group at Max Planck Institute for Chemical Ecology, Jena, Germany and are available from the corresponding author on reasonable request.

7,11-HD:

(7Z,11Z)-Heptacosa-7,11-diene

7,11-ND:

(7Z,11Z)-Nonacosa-7,11-diene

CG:

Crystal growth ordering

CH503:

3-O-Acetyl-1,3-dihydroxy-octacosa-11,19-diene

cVA:

11-cis-accenyl acetate

Da: Dalton DHB:

2,5-Dihydroxybenzoic acid

GC-MS:

Gas chromatography – mass spectrometry

LDI:

Laser desorption ionization

LiDHB:

Lithium 2,5-dihydroxybenzoate

MALDI-TOF:

Matrix-assisted laser desorption/ionization – time of flight MS: Mass spectrometry

MSI:

Mass spectrometry imaging

SEM:

Scanning electron microscope

Financial support from the Max Planck Society for instruments is gratefully acknowledged. We would like to thank Frank Steiniger from Elektronenmikroskopisches Zentrum in Jena, Germany for his help with SEM images and also Sybille Lorenz and Kerstin Weniger, Anne Späthe, all from MPI-CE, for measuring samples on GC-MS. We would like to thank Emily Wheeler, Boston, for editorial assistance.

Heading

2-D surface distribution of sex pheromones within the whole Drosophila fly by mass spectrometry imaging.

Financial support instrumentation, supply, and salary was provided by the Max Planck Society.

Authors and Affiliations

1. Max Planck Institute for Chemical Ecology, Hans-Knöll-Strasse 8, D-07745, Jena, Germany

   Filip Kaftan, Markus Knaden, Bill S. Hansson & Aleš Svatoš

2. Chair for Bioinformatics, Friedrich Schiller University Jena, Q2 Ernst-Abbe-Platz 2, D-07743, Jena, Germany

   Purva Kulkarni & Sebastian Böcker

Contributions

FK designed and performed (MA) LDI experiments. FK and AS wrote the manuscript. PK recalibrated MSI datasets and generated 2-D ion intensity maps. AS, MK, BSH and SB revised the manuscript. All authors read and approved the final manuscript.

Corresponding authors

Correspondence to Filip Kaftan or Aleš Svatoš.

Ethics approval and consent to participate

Not applicable.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

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