Lizard Survey to Determine the Effects of Parasite Load on Lizard Survival

A monthly capture-mark-recapture (CMR) survey of T. viridipunctatus was conducted between July and November in 2008 and 2009 at Cape Jinshan on the northeastern coast of Taiwan (25°13′34″N, 121°38′55″E). The lizards were captured by hand at night along a 500-meter transect. All captured individuals were uniquely tagged by toe clipping, sexed, and aged, and the number of the trombiculid mites (Leptotrombidium sp.) on each lizard was counted before they were released back to the population. Only adult lizards (totally 1104 individuals) were included in the survival analysis to match the separate samples used in our analyses of heterozygosity-fitness correlations in adult lizards.

Two methods were conducted to evaluate the effect of parasites on survival of adult lizards during the breeding season. First, we used Spearman correlations to check the association between maximum capture interval (in month) and the mean parasite load (the mean number of mites from each capture of each lizard). We then used the Cormack-Jolly-Seber (CJS) model implemented in program MARK [34], [35] to estimate the survival of adult lizards as a linear function of mean number of trombiculid mites. The CJS model estimates two parameters: survival (φ) and recapture probability (p). Although φ is the probability that any given individual will have remained in the population and survived through a specific time period, and thus cannot be used to distinguish between mortality and emigration, our study site is surrounded by urban areas and ocean, making successful emigration unlikely. The time and sex dependency of survival and recapture probability were first evaluated with Akaike's Information Criterion, corrected for small sample sizes (AIC_c), which suggested that survival is constant (φ.) or sex-varying (φ_sex) and that recapture probability is time- and sex-varying (p_sex×t; Table S1). We used these two models as base models (φ. p_sex×t and φ_sexp_sex×t) and constructed four additional models to test the effects of mites on the T. viridipunctatus survival functions: sex-varying intercepts and slopes of mean number of mites, sex-varying intercept and a constant slope of mean number of mites, a constant intercept and sex-varying slopes of mean number of mites, and constant intercept and slope of mean number of mites (Table 1). The fit of the more complex base model (φ_sexp_sex×t) was assessed with C? (≈χ²/df); a C? close to 1 indicates perfect model fit, and a C? smaller than 2 usually suggests a good fit. We used the three estimates of C? implemented in MARK to assess model fit: (1) C? from the program RELEASE, which provided an estimate of C? = 0.82 (RELEASE does not provide standard errors); (2) median C? = 1.04±0.02 (± SE); and (3) bootstrap C? = 1.57±0.02. All three estimates suggest a fairly good model fit. In addition, we visually assessed the distribution of the residuals using the residual deviance plot, which suggested that the residuals are randomly distributed around zero. Model goodness of fit cannot be directly assessed when individual covariates are incorporated in the CJS models. However, given that the base model had a good fit, we were able to test the effects of mite parasitism on lizard survival using likelihood ratio (LR) tests (i.e., determine whether the models with mean number of mites as a covariate significantly improved the model fit from the base models).

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Table 1. Model selection from six candidate survival functions.

https://doi.org/10.1371/journal.pone.0056720.t001

Lizard Sampling for Correlations among Individual Heterozygosity, Parasite Load, and Scalation Asymmetry

The toe-clipping method used in the long-term survey made it difficult to quantify scalation asymmetry (the scalation asymmetry scores of the toes are included as part of the asymmetry measure), one of the two fitness traits used in our HFC study. To obtain a sample of lizards with intact toes, we conducted a separate sample collection. To ensure that this sampling did not interfere with the survival estimates, we collected 140 adult lizards (78 males and 62 females) from a nearby location in July 2008. Although this sampling could potentially lower the lizard population size, the 2008–2009 survival estimates were based on lizards marked after this sampling was conducted. Compared to the estimated population sizes of 1,122 in 2008 and 1,066 in 2009 during these months (minimum number alive), a sample of 140 individuals was likely to represent only 12–13% of the population. In addition, we conducted the sampling approximately 100 meters from the survey transect to ensure that we removed only individuals at the boundary of the population for which we were estimating survival. We used only adult lizards without autotomized tails in this sampling to control for the potentially confounding effects of lizard body condition on mite infestation.

Individual Heterozygosity

Genomic DNA was extracted from lizard muscle tissues using a modified LiCl method [36]. Ten microsatellite loci [37] were evaluated to estimate individual heterozygosity (Table S2). The polymerase chain reactions (PCRs) were set up in a volume of 10 µl containing 50–100 ng genomic DNA, 1× PCR buffer (PROMEGA), 0.15–0.2 µM each forward and reverse primers, 2.5 mM MgCl₂, 0.2 mM dNTP, and 0.25 U Taq DNA polymerase (PROMEGA). PCR was carried out under standard conditions, with modifications for each locus [37]. The PCR products were electrophoresed in a MegaBASE™ 1000 autosequencer (Amersham Bioscience, New Jersey, USA) with size marker ET-400 (Amersham Bioscience New Jersey, USA). Alleles were scored manually in GENETIC PROFILER version 2.2 (Amersham Bioscience, New Jersey, USA). Tests for departure from Hardy-Weinberg equilibrium and linkage disequilibrium between pairs of loci were performed using Arlequin ver. 3.5 [38]. Two of the 10 microsatellite loci were found to be out of Hardy-Weinberg equilibrium. However, the analyses of the data with either eight or 10 microsatellite loci gave similar results. Therefore, we reported only the results based on all 10 microsatellite loci.

Individual heterozygosity was initially evaluated by three different approaches: standardized mean d-squared (standardized d²), internal relatedness (IR), and heterozygosity weighted by locus (HL). Standardized mean d² is defined as squared distance divided by the maximum value observed on that locus, and then averaged across loci [39]. HL [40], an estimate of parental relatedness, is modified from the widely applied IR [41] but tends to outperform the latter. Because HL and IR are highly correlated (r² = 0.96) in this study, only HL was retained in the following analyses. Because standardized mean d² was considered less informative in recent studies [6], [13], we accept HFCs only when the results based on standardized mean d² and HL are congruent.

Parasite Load

Parasite load, i.e., the number of parasites on a host, was measured by immediately counting the number of trombiculid mites attached to each individual lizard (Figure 1). These mites are relatively large in size (∼400 µm) and bright red in color. They attach themselves tightly to gaps between the ventral scales using their jaws and are therefore visible as a pattern of discrete spots. The morphological and behavioral characteristics of these mites allowed for an accurate count of parasite load. The parasite load was quantified using an identical protocol in the 2008–2009 survey and the separate sample of 140 lizards, and mean parasite load was calculated for individuals who were captured multiple times during the survey.

Scalation Asymmetry

Scalation asymmetry was measured for the separate sample of 140 lizards by summing the absolute difference in scale numbers between the left and right sides across the chin shields, supralabials, infralabials, supraciliary scales, and supraocular scales in the head region and the subdigital lamellae of all fingers and toes of the limbs. The raw asymmetry scores ranged between 0 to 3 in the head region and 1 to 14 in the limbs. Therefore, we converted the limb asymmetry scores to a 0–3 scale using the following equation: (limb asymmetry score-1)/4.33. We added the head and normalized limb asymmetry scores to produce an overall asymmetry index that ranges from 0 to 6.

Tests of Single-locus Effects

Single-locus effects or local effects could lead to spurious HFCs [42], [43], [44]. This alternative mechanism should be carefully evaluated before testing HFCs. Here, we evaluated the potential for single-locus effects in the three steps. First, we assessed the homology of the microsatellite flanking sequences to published Squamata expressed-sequence tags (ESTs). We performed a BLAST search of the flanking regions of each microsatellite locus (sequences available in GenBank; accession numbers are given in Table S2) against the green anole (Anolis carolinensis) EST database using the NCBI BLAST suite (http://blast.ncbi.nlm.nih.gov/). We did not find any homologous ESTs between A. carolinensis and the flanking sequences of the 10 microsatellite loci. Therefore, the loci we used in this study were not likely to be in functional genes.

Secondly, cryptic population structure is known to produce spurious HFCs [45]. This possibility could be ruled out by testing for heterozygosity differences among populations, or in our case for a single population, to provide evidence that the population is unstructured [46], [47]. The software STRUCTURE 2.3.4 [48] was used to implement Bayesian MCMC inference of a posteriori genetic clusters and detect any cryptic genetic structure in the assumed a priori populations (Mank and Avise 2004). The number of assumed genetic clusters (K) was set from 1 to 10, and 15 runs were performed for each K with 200,000 MCMC iterations (initial 20,000 iterations discarded as burn-in). The results for cluster size K = 1 (LnP(D) = −6621.9) were significantly better than those for K = 2 (LnP(D) = −6910.8, P = 0.009) or any higher K values. These results demonstrate that the Jinshan Cape lizard population is unstructured.

Finally, a formal statistical test of single-locus effects was conducted [49]. We performed the F ratio test to determine whether multiple regression incorporating specific effects from each locus (i.e., using heterozygosity at each locus as one predictor, for a total of 10 predictors) explains more variance in a fitness trait than a simple regression using only one predictor, multilocus heterozygosity (MLH). The heterozygosity at each locus was scored as 0 for homozygous and 1 for heterozygous. Missing data were replaced with the mean heterozygosity for that locus [47], [49]. We used the parasite load as the fitness trait in this test because its relationship with lizard fitness (i.e., survival) was formally tested in this study. We log-transformed the parasite load prior to the regression analyses to improve data normality. The results suggest that single-locus multiple regression did not explain more variance in parasite load than did MLH simple regression (F_9,129 = 0.482, P = 0.88). Therefore, single-locus effects were not found in this study.

Tests of HFCs

The two fitness-related traits, parasite load and asymmetry index, were not correlated (Spearman correlation, P = 0.62). Hence, their relationships with individual heterozygosity (standardized mean d² and HL) were analyzed separately. The parasite load and asymmetry index data were non-normally distributed. Therefore, the associations between heterozygosity and parasite load or asymmetry index were tested with Spearman correlations. To investigate sex-specific HFCs, we performed Spearman correlations for the whole population, as well as for males and females separately. Because individual heterozygosity increases with standardized mean d² and decreases with HL, the correlations between these two measures and a fitness trait should be in the opposite directions (e.g., a negative correlation between standardized mean d² and parasite load and a positive correlation between HL and parasite load both suggest a positive HFC). Sex differences in parasite load and asymmetry index were examined using Kruskal-Wallis test. All statistical analyses were performed in SAS 9.2.

Ethics Statement

The lizard handling and processing protocols were approved by the Institutional Animal Care and Use Committee of National Taiwan Normal University (Permit No. 101007). No other specific permits were required because the field studies were not conducted in a protected area, and the sampling did not involve endangered or protected species.

Lizard Survival and Parasite Load

Maximum recapture interval (in month) of the 1104 adults represented a negative correlation against parasite load (r_s = −0.13, P = 0.0013; Figure 2A), indicating an increase of the mites decreased the probability of the lizard to survive for a long period. Mean number of mites as a covariate for monthly survival of adults in T. viridipunctatus was well supported based on the AIC_c and LR tests (models 3–6; Table 1). The CJS models with sex-varying slopes of the mean number of mites in lizard survival functions did not significantly improve model fit compared to the models with a constant slope (LR tests: model 3 versus 5, Chi.-sq. = 0.002, P = 0.96; model 4 versus 6, Chi.-sq. = 1.913, P = 0.17), suggesting that the effects of mites on lizard survival were similar in males and females. In fact, all four models with mean number of mites as a covariate for adult survival (models 3–6; Table 1) estimated negative slopes for mean number of mites (estimated β ± SE: models 3&4, −0.032±0.007; model 5 males, −0.032±0.007; model 5 females, −0.032±0.007; model 6 males, −0.047±0.016; model 6 females, −0.025±0.008), indicating that survival decreased with increasing parasite load for all adult lizards (Figure 2B).

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Figure 2. Maximum recapture interval (A) and monthly survival rate (B) of Takydromus viridipunctatus against parasite load.

This estimation was derived from 1104 adults during the breeding seasons of 2008 and 2009. The maximum recapture interval (in month) decreased with increasing mean parasite load (the mean number of mites of each capture), where the size of shaded circles is in proportion to the sample size (A). The solid and dashed lines (B) denote estimated survival with the 95% confidence intervals, indicating that monthly survival rate decreased with increasing mean number of mites. The covariate plot is based on model 3 in Table 1 and its maximum likelihood estimates, logit(φ) = 1.614±0.318 (SE)−0.032±0.007×(mean number of mites).

https://doi.org/10.1371/journal.pone.0056720.g002

Individual Heterozygosity and Parasite Load

The 140 lizards collected in July 2008 varied widely in parasite load, ranging from 0 to 130, with a median of 12.5 mites per host. The standardized mean d² and parasite load for the whole population were negatively correlated (r_s = −0.26, P = 0.0019, n = 140), and this correlation was driven by the males (males: r_s = −0.37, P = 0.0005, n = 78; females: P = 0.72, n = 62; Figure 3A and 3C). However, HL and the parasite load of the whole population were not correlated (P = 0.97, n = 140), which was a result of the opposite correlation directions between males and females (males: r_s = 0.20, P = 0.08, n = 78; females: r_s = −0.26, P = 0.04, n = 62; Figure 3B and 3D). When the results from the standardized mean d² and HL were combined, the male lizards showed a consistent pattern in which decreased parasite load was associated with increasing individual heterozygosity (approximately 14% and 4% of the variance in parasite load was explained by the standardized mean d² and HL, respectively). The relationships between individual heterozygosity and parasite load for female lizards, as well as for the whole population, were inconclusive. The male-only correlation between individual heterozygosity and parasite load was not likely to be a result of a higher parasitism risk for males because males and females had similar parasite loads (Kruskal-Wallis test, χ² = 0.88, P = 0.35). In addition, both sexes had a similar frequency distribution of parasite load, with a median of 8 (25^th–75^th percentile = 2–52) for males and 18.5 (25^th–75^th percentile = 4–46) for females.

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Figure 3. Correlations between individual heterozygosity and parasite load in Takydromus viridipunctatus.

The parasite load (i.e., the number of the trombiculid mites Leptotrombidium sp. on each lizard) increased with decreasing standardized mean d² (A) and increasing HL (B) in male T. viridipunctatus. The parasite load did not change with the standardized mean d² (C) but decreased with increasing HL (D) in female T. viridipunctatus. Each circle denotes one individual.

https://doi.org/10.1371/journal.pone.0056720.g003

Individual Heterozygosity and Scalation Asymmetry

The standardized mean d² and scalation asymmetry index for the whole population were not correlated (P = 0.25, n = 140). However, males with increasing standardized mean d² tended to have lower asymmetry (males: r_s = −0.20, P = 0.08, n = 78; females: P = 0.98, n = 62; Figure 4A and 4C). In contrast, HL and scalation asymmetry index were positively correlated for the whole population, as well as for either males or females alone (whole population: r_s = 0.22, P = 0.008, n = 140; males: r_s = 0.19, P = 0.10, n = 78; females: r_s = 0.29, P = 0.02, n = 62; Figure 4B and 4D). When the results of the standardized mean d² and HL were combined, male lizards showed a consistent relationship between decreased scalation asymmetry and increasing individual heterozygosity (approximately 4% of the variance in scalation asymmetry was explained by the standardized mean d² and HL). The relationships between individual heterozygosity and scalation asymmetry for female lizards, as well as for the whole population, were inconclusive. The male-only correlation between individual heterozygosity and scalation asymmetry was not likely to be a result of higher asymmetry in males because males and females exhibited similar asymmetry index values (Kruskal-Wallis test, χ² = 0.97, P = 0.32). In addition, both sexes had a similar asymmetry index frequency distribution, with a median of 2 for both males (25^th–75^th percentile = 2–3) and females (25^th–75^th percentile = 1–3).

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Figure 4. Correlations between individual heterozygosity and scalation asymmetry in Takydromus viridipunctatus.

The scalation asymmetry increased with decreasing standardized mean d² (A) and increasing HL (B) in male T. viridipunctatus. The scalation asymmetry did not change with standardized mean d² (C) but increased with increasing HL (D) in female T. viridipunctatus. Each circle denotes one individual.

https://doi.org/10.1371/journal.pone.0056720.g004