Ethics Statement

All experimental procedures were approved by the Institutional Animal Care and Use Committee at the University of Texas at Austin (protocol #07110101).

Paradigm

All experiments were conducted with sexually mature wild caught or progeny of wild caught female X. nigrensis maintained at University of Texas Brackenridge Field Laboratories in Austin, Texas. Immediately prior to the behavior trials, as a control we measured a proxy for circulating estradiol to account for potential influences of estrogen on behavior or localized gene expression patterns through a non-invasive waterborne assay (see below). We followed established behavioral measurements, dichotomous choice paradigm, and natural lighting conditions to assess preference in this species [30]. Briefly, the behavioral testing arena (120 cm×30 cm×48 cm aquarium) was divided into five 24 cm zones. One zone at each end of the tank contained stimuli fish behind a barrier. The three remaining subsections are open to the focal female and consisted of a middle “neutral” zone with an “association” zone adjacent to each stimulus. Females were acclimated for 5 minutes in the center (neutral region) of the experimental tank and allowed to interact with either end stimuli (behind UV-transparent plexiglass partitions) for 30 minutes, with stimuli switched after 15 minutes to disassociate female preference for a specific stimulus from side bias.

For each behavioral trial we recorded (i) the number of female glides (a display wherein the female initially orients towards the stimulus, turns and swims away, but then returns to the initial stimulus-facing position; glides are considered a proxy for receptivity and can precede copulatory events in X. nigrensis and related species [45]–[47]), (ii) the overall locomotor activity of each female by counting transits (number of times a female swims into a central neutral zone in the tank), and (iii) association bias. Association bias is defined as the proportion of time spent with stimulus a (i.e. in association zone adjacent to stimulus a) where time spent with stimulus a > stimulus b. Since females can have similar association biases but vary in the frequency of behaviors (e.g. glides and transits), we calculate a composite preference score that encompasses both time and behavior (preference score (PS)  =  association bias + log [(1 + receptivity displays towards the biased stimulus)/total transits]) as in [30], [32], [48]. As the PS involves a log transformation of our behavioral measures, more positive PS indicates the female showed both a relatively higher bias in association time and glides toward one stimulus (normalized by general locomotor activity); whereas more negative PS indicates the female generally showed relatively little bias in association time and/or behavior.

Females in Experiment 1 (egr-1 quantification) were subjected to one of three conditions: a mate choice context (one large and small male, LS, n = 10), two size-matched females (FF, n = 10), or to an asocial control (AA, n = 10) wherein the focal female was placed in the experimental tank without any stimuli at either end. All size-matched stimuli differed by no more than 1 mm standard length. We conducted Experiment 2 (neuroserpin quantification) independently to determine if we saw similar localization patterns and preference behavior associations between a general activity marker (egr-1) versus our more context-specific marker (neuroserpin). As we previously demonstrated an association between mate preference and whole-brain neuroserpin expression [30], [31], we expanded the social exposure paradigm to include presumed levels of complexity (see below). Females in Experiment 2 (neuroserpin quantification) were subjected to one of five conditions: two size-matched large males (LL, n = 10) with one male behind a UV pass barrier and the other behind a UV blocking filter, one large and small male (LS, n = 13), two size-matched small males (SS, n = 7), two size-matched females (FF, n = 12), or collected from their home tank (HT, n = 6), a treatment serving as an asocial control context (females are housed in isolation). Home tank females underwent the same pre-testing estradiol measurements as females exposed to the other contexts but were then returned to their home tanks for 30 min. prior to sacrifice. We selected our three male-exposure conditions to represent a gradient in mate choice complexity with the LL treatment context representing a relatively complex mate preference environment (two preferred phenotypes varying in UV ornamentation), and the LS and SS treatment contexts representing a simple and minimum mate preference environment, respectively. Females can both see and prefer males with UV ornamentation [28]. Therefore we used UV pass and blocking filters in the LL trials to allow females to discriminate between two attractive males by a secondary sexual characteristic other than size in this more complex condition.

Females were isolated at least two weeks before behavioral testing to ensure sexual motivation. Each female was pre-tested twice with large/small stimuli prior to context assignment to ensure similar baseline preference responses across experimental contexts. Females in Experiment 1 (large/small, female/female, and asocial conditions) or Experiment 2 (large/large, large/small, small/small, female/female, home tank condition) showed no significant differences in pre-test preference trials (egr-1 ANOVA, PS: p = 0.122; neuroserpin, ANOVA, PS: p = 0.992).

We identified “high” performing (> median) females for each behavior of interest (preference score, transits, or glides) and compared their gene expression in each brain region (see below) with females identified as “low” performing (< median). For context specific comparisons, we examined the relationship between gene expression and behavior in each region for females exposed to males (large/large, large/small, and small/small) relative to female-exposed females (FF). We subsequently examined the unique covariation patterns between brain regions for each male-exposed environment (large/large, large/small, or small/small).

Estradiol Measurements

We quantified estradiol levels for all females through a non-invasive waterborne assay following an established protocol for teleosts [49]–[51] and validated in our focal species [48]. Briefly, females were placed in a 250 mL glass beaker containing 150 mL of reservoir water (treated tap water used for home and experimental tank) for one hour prior to behavior trials. Estradiol was extracted from the water using C18 Solid Phase Extraction columns (Sep-Pak Plus C18 cartridge 55–105 lm; Waters Corporation, Milford, MA) and measured on a Correlate-EIA 17β-estradiol Enzyme Immunoassay Kit (Assay Designs) according to manufacturer's protocol. Hormone samples were run on three 96-well EIA assay plates: inter-assay CV was 6.5% and intra-assay CV was 1.9%.

Tissue Processing and in situ hybridization

Females in each experiment were decapitated within 30 seconds of the end of the behavior trial and brains were frozen on dry ice. We stored tissue at −80°C until sectioning at 16 µm onto serial series. Tissue fixation parameters, probe synthesis, and in situ hybridization conditions were modified from established protocols [8], [52]. For Experiment 1 (egr-1 quantification), we used only a digoxigenin (DIG)-labeled probe. For Experiment 2 (neuroserpin quantification), we used DIG-labeled probe for one series and S35-labeled probe for another series. Each series was processed simultaneously to minimize technical variation. Sense riboprobes showed negligible to no expression (Figure S1). Please see Methods S1 for detailed process parameters.

Gene expression quantification

Using a X. helleri brain atlas for reference and terminology [53], we identified and quantified DIG-labeled riboprobe expression in 10 brain regions (Table 1). These brain regions include putative teleost homologs [16], [17], [54], [55] for nodes in the social behavior network (SBN [15], [16]), reward system (the mesolimbic dopaminergic reward pathway [56]), and other regions. While the tetrapod homology of some teleost brain regions are difficult to determine due to different neural developmental trajectories [55], in the current study we follow designations established from other studies focusing on homologies [16], [17], [55]. After tissue processing final sample sizes for Experiment 1 (egr-1 quantification) were: large/small, n = 6; female/female, n = 7; asocial, n = 10. For Experiment 2 (neuroserpin quantification) final sample sizes were: large/large, n = 10; large/small, n = 10; small/small, n = 5; female/female, n = 9; home tank, n = 5.

Statistics

All statistics were performed in SPSS (ver. 18) and the network statistics were conducted using Ucinet [62]. We used a t-test to examine context-wide behavioral and gene expression differences between individuals expressing high versus low behaviors in each treatment condition and a Benjamini-Hochberg correction [63] for multiple hypothesis testing. To assess relationships between individual variation of preference behavior, gene expression, or estradiol levels we used Pearson's correlation when the data was normal and Spearman correlation when data was non-normal (glides and transits) and corrected for multiple hypothesis testing as above. We calculated effect sizes and conducted a post-hoc power analysis to calculate achieved power (1 – β error probability) using G*Power 3.1 computer software [64]. As the effect size for correlation analyses is the absolute value of the correlation coefficient, we just report the correlation coefficient for simplicity. For the correlation analyses, we designate “high”, “medium”, and “low” effect size boundaries as 0.5, 0.3, and 0.1, respectively, as in [65], [66]. For significant correlations between gene expression and preference score, we additionally ran a randomization test on correlation coefficients with replacement 10⁵ times using freeware provided by Dr. David C. Howell (http://www.uvm.edu/~dhowell/StatPages/Resampling/Resampling.html#Return1). This process allows us to examine the probability that the observed coefficient correlations were due to chance. Randomization with replacement holds the behavioral measure constant and randomly pairs the OD of a brain region to obtain a correlation coefficient. After multiple runs (10⁵), we generated a distribution of correlation coefficients for each brain region and behavioral measure. By comparing the observed correlation coefficient against the generated distribution, we rejected the null hypothesis that r = 0 when the observed value had less than 5% probability of occurring.

We directly compared correlation coefficients by doing a Fisher r-to-z transformation and then use a Z-test to assess brain region expression consistency between egr-1 and neuroserpin. Due to uneven sample sizes across experiments we calculated effect sizes and achieved power as above when analyzing consistency of expression between experiments. We calculate effect size (q) following standard methodology (difference between the two Fisher-z-transformed correlation coefficients) and designate “high”, “medium”, and “low” effect size boundaries as 0.5, 0.3, and 0.1, respectively, as in [65]. We considered consistent expression across both experiments if we observed non-significant differences between the correlation coefficients across the two experiments for the male-exposed and female-exposed environments.

To begin to identify and characterize a network of brain regions associated with female mate preference, we utilized network analyses [67], [68]. Specifically we examined coordinated patterns (i.e. pairwise correlations) of neuroserpin expression across all brain regions, by converting all Benjamini-Hochberg corrected correlations of neuroserpin expression between regions into binary values in an association matrix (1 =  significant correlation, 0 =  non-significant). We then analyzed (i) the degree centrality of brain regions in each treatment context (large/large, large/small, small/small, female/female, home tank), and (ii) the density of these networks. Due to small sample size, we did not analyze egr-1 network expression patterns.

Degree centrality is a way to assess how connected a node is in a network [67], and here we evaluate it by assessing the number of significant correlations between focal brain regions. The assumption is that a brain region with a high number of correlations with other regions may have a more central role in preference dynamics. Degree centralities for each node in each network were calculated in Ucinet and then compared to other nodes in the same network using a Wilcoxon Rank Sum test in SPSS. For each exposure condition, we calculated effect size and achieved power as above. We used an established formula to calculate effect size (d) for nonparametric analyses (difference between the means divided by the standard deviation [65]). We designate “high”, “medium”, and “low” effect size boundaries as 0.8, 0.5, and 0.2, respectively, as in [65].

We also evaluated network density [67] to assess the complexity of the neuroserpin expression response during preference using a t-test. Density is evaluated as the number of unique correlations in each of the male exposed contexts (large/large, large/small, small/small) by removing overlapping correlations found in the controls (FF or HT).

Female preference

As reported in previous studies [27], [30], [32], [45], females preferred to associate with large males over small males in both Experiment 1 (egr-1 quantification, large males: 955.5±109.6 sec, small males: 578±116.4 sec, t = 2.3, n = 6, p = 0.039) and Experiment 2 (neuroserpin quantification, mean association time ± SE with large males: 1160±78.1 sec, small males: 373.6±50.8 sec, t = 8.4, n = 10, p = 1.1 * 10⁻⁷) experiments. In Experiment 1 (egr-1 quantification), females exposed to an empty stimulus environment (AA) displayed a tendency for a side bias (left side association time: 571.8±75.9 sec, right side: 790.7±76 sec, t = −2.0, n = 10, p = 0.056). Females exposed to large/small (LS) conditions in Experiment 1 (egr-1 quantification) had significantly higher preference scores than females exposed to the asocial conditions (AA, t = 2.3, p = 0.037, Figure 1A), while females in all social exposure contexts of Experiment 2 (neuroserpin quantification) exhibited similar ranges of preference scores (F = 1.92, p = 0.14, Figure 1B).

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Figure 1. Female preference behavior.

Behavioral preference scores for each individual in (a) Experiment 1 (egr-1 quantification) and (b) Experiment 2 (neuroserpin quantification) by treatment context. Gray horizontal line is the median with standard error. Black and white circles represent high (> median) and low (< median) preference score females, respectively. *, p<0.01.

https://doi.org/10.1371/journal.pone.0050355.g001

DIG quantification validation

We conducted in situ hybridization of neuroserpin expression (Experiment 2) on 39 females using both non-radioactive (digoxigenin, DIG) and radioactive (S35) methods on serial sections. The S35-labeled riboprobes provided validation of the DIG-labeled approach as evidenced by (i) a significant positive correlation between the two quantification methods (r = 0.351, p = 0.008, Figure S2A), (ii) consistent context-specific neuroserpin expression patterns in Dm by both methods for high (> median) relative to low (< median) performing females for preference score, glides and transits (Table S1), and (iii) significant correlations between neuroserpin expression in Dm and preference score for male-exposed females in both approaches (Figure S2B).

Localized gene expression and preference behavior

To quantify DIG-labeled gene expression in 10 different regions we measured the optical density (OD) within each region (see methods). There were no significant across treatment differences in either egr-1 or neuroserpin expression for any brain region after correcting for multiple comparisons (Figure S3). Within exposure context, however, there were clear differences in neuroserpin expression between females expressing a high versus low preference score (male exposed or female/female (FF)) within three forebrain (Dm, Dl, POA) and one midbrain (HV) region (Figure 2, Table S2). Male-exposed females (small/small (SS), large/small, and large/large (LL)) but not FF females (Table S2) with high preference scores had significantly higher neuroserpin expression than low preference score females in each of these brain regions (Dm, t = 3.284, p = 0.003; Dl, t = 2.91, p = 0.008; POA, t = 3.292, p = 0.003; HV, t = 2.489, p = 0.021, Figure 2, Table S2). The difference in neuroserpin OD in HV was not significant after a multiple hypothesis correction.

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Figure 2. Neuroserpin expression in male-exposed females.

(A) Significant differences in neuroserpin expression of male-exposed females (large/large, large/small, small/small) between groups of high (black) and low (white) preference score females measured in Dm, Dl, POA, and HV. Bars represent standard error. **, p<0.01; *, p<0.05. (B–D) are representative images of a high-preference female (preference score  = 0.4) for Dm, Dl, POA, respectively. (E–F) are representative images of a low-preference female (preference score  = −0.91) for Dm, Dl, POA, respectively. Scale bar is 25 microns.

https://doi.org/10.1371/journal.pone.0050355.g002

Using S35-labeled neuroserpin riboprobes, we measured expression in Dm and found a significantly greater number of neuroserpin positive cells in high preference females over females displaying low preference (mean ± SE: high preference score  = 309.56±22.85, low preference score  = 213.89±18.04, t = 2.079, p = 0.003) in only male-exposed females (Table S1). There were no significant differences in neuroserpin expression with either DIG or S35 labeled riboprobes in any context (male exposed or FF) between high versus low performing females for glides and transits (Tables S1 & S3). Due to small final sample sizes we did not analyze egr-1 expression differences between high versus low preference females.

Individual variation in gene expression and behavior (region and context specificity)

Of the four brain regions that showed differences in neuroserpin OD between high and low preference females, three exhibited significant positive correlations between individual variation of female preference score and neuroserpin expression in male-exposed females only: Dm (n = 25, r = 0.522, p = 0.007, Figure 3a), Dl (n = 25, r = 0.501, p = 0.011, Figure 3b), and POA (n = 25, r = 0.479, p = 0.015, Figure 3c) but not HV (n = 25, r = 0.368, p = 0.07). Randomization tests show that the relationships seen between neuroserpin expression and preference score in Dm, Dl and POA are not likely due to chance (p<0.02, Table 2). We obtained similar results when quantifying preference score and neuroserpin Dm expression with the S35 quantification method (n = 25, r = 0.405, p = 0.049, Figure S2B). Egr-1 expression was correlated with preference score in male-exposed females in Dm (n = 6, r = 0.829, p = 0.041, Figure 4), a trend in Dl (n = 6, r = 0.797, p = 0.057) but not in POA (n = 6, r = −0.003, p = 0.994), while exhibiting no correlation with mate preference in any other context (Table S4). Randomization test indicate that the relationship between egr-1 expression and preference score in Dm is also not likely due to chance (p<0.05, Table 2). While we observed a significant correlation between Pit neuroserpin expression and preference score (Table 2), we did not observe expression differences in this region between high and low PS females (Table S2). These relationships were mate preference-specific, as neither egr-1 nor neuroserpin expression were significantly correlated with other behaviors (transits or glides) in Dm, Dl, or POA in any condition (Table S5). To assess whether these relationships were driven by the size asymmetry in the large/small context, we removed the large/small context from the analyses and observed that high preference score females in the size-matched male conditions still had significantly higher neuroserpin expression than low preference score females in the candidate regions (LL & SS, Dm: t = 5.5 p = 0.0001; Dl: t = 5.6 p = 0.0001; POA: t = 5.1, p = 0.0002), as well as significant correlations between preference score and neuroserpin expression (Dm: n = 15, r = 0.678, p = 0.005; Dl: n = 15, r = 0.7, p = 0.003; POA: n = 15, r = 0.7, p = 0.003). In contrast, we do not see a significant correlation between preference score and neuroserpin expression in the same brain regions in the size matched female/female context. Finally, there were no significant correlations between circulating estradiol levels and preference score, glides, transits, or gene expression in any brain region for any treatment context after correcting for multiple hypothesis testing (Table S6). This suggests that differences in circulating estradiol levels between individuals are an unlikely explanation for our observed gene expression patterns with mate preference behavior.

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Figure 3. Individual variation of preference score and neuroserpin expression.

Significant correlations between individual variation in preference score and neuroserpin expression in (a) Dm, (b) Dl, and (c) POA. Triangles, diamonds, and squares represent LL, LS, and SS exposed females, respectively.

https://doi.org/10.1371/journal.pone.0050355.g003

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Figure 4. Individual variation of preference score and egr-1 expression.

(a) Significant correlation between individual variation in preference score and egr-1 expression in Dm. Representative images of egr-1 expression in Dm for two individuals with a preference score of (B) 0.66 and (C) −0.26. Scale bar is 25 microns.

https://doi.org/10.1371/journal.pone.0050355.g004

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Table 2. Gene expression (egr-1, neuroserpin) correlated with preference score in each of the 10 brain regions (first column) within and between experiments for female exposed to males or females.

https://doi.org/10.1371/journal.pone.0050355.t002

Egr-1 and neuroserpin regional expression consistency related to behavior

Egr-1 and neuroserpin were expressed in all examined regions in all contexts (Figure S3). We found no significant differences in correlations in region-specific gene expression and preference score across experiments, although our effect size was relatively low for detecting differences in Cb, GC, and Vv brain regions (Table 2). For the male-exposed environments, both egr-1 and neuroserpin showed consistent expression patterns, including consistent positive correlations within Dm and Dl (Table 2). Similarly, both genes showed consistent patterns in the female exposed environments, for all brain regions examined in the current study (Table 2). Effect size calculations showed that overall we achieved medium to high effect sizes in the male (average effect size: 0.421±0.22) and female (average effect size: 0.385±0.48) exposed contexts (Table 2).

Context-specific expression networks

Looking at within network dynamics, candidate regions associated with mate preference (Dm, Dl, and POA) had a significantly higher degree centrality relative to the other seven brain regions in females exposed to males (Z = 2.44, p = 0.015 (large/large); Z = 2.34, p = 0.019, (large/small); and Z = 2.59, p = 0.009, (small/small); Table 3) whereas females exposed to females (p = 0.55) or asocial conditions (p = 0.35) showed no significant difference. For instance, in the large/large context, the degree centrality of Dm (0.33), Dl (0.44) and POA (0.57) was 3–5 times greater than the average of the other brain regions (mean degree centrality  = 0.158; Table 3). Post-hoc power analyses show that overall the effect size was high (Table 3).

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Table 3. Degree centrality of neuroserpin by social context for each brain region, in each treatment group for females used to localize neuroserpin.

https://doi.org/10.1371/journal.pone.0050355.t003

To compare across networks we assessed the density of the networks in each male-exposed condition. We observed one unique male exposure correlation that was constant across all three male exposure contexts (Dm with POA) while others appeared only in specific male environments (e.g. Dm with Vv in the presence of large males (LL, LS) but not in small male only conditions (SS), Figure 5). Furthermore, there was a significantly higher network density (i.e. total number of unique significant correlations between regions) for females exposed to LL relative to LS (t = 3.23, p = 0.0026) and SS (t = 3.52, p = 0.0028) male contexts.

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Figure 5. Neuroserpin expression network by context.

Unique significant positive pairwise correlations relative to FF and HT females in neuroserpin expression between brain regions (lines) in A) LL, B) LS, and C) SS exposed females. Brain regions bolded in the schematic sagittal section are those associated with mate preference identified in this study.

https://doi.org/10.1371/journal.pone.0050355.g005