Ethics statement

The work met the Spanish legal requirements about animal welfare (approval identification: PAI06-0018; Consejería de Medio Ambiente, Junta de Comunidades de Castilla La Mancha; JCCM) and was supervised by the veterinary staff of Instituto de Investigación en Recursos Cinegéticos (Ciudad Real, Spain).

Study model

Red-legged partridges show conspicuous traits (Fig. 1) with a slight sexual dichromatism (males are redder) [27]. Red pigmentation in the head is produced by carotenoids and is positively correlated to cell-mediated immune response and size-corrected body mass (i.e., “body condition”) [28], [29]. It is also sensitive to food restriction [29] and predicts resistance to oxidative damage after an experimental immune challenge [30]. Female partridges doubled their reproductive investment (i.e., clutch size) when the redness of their mates is experimentally intensified (C Alonso-Alvarez, unpublished). Positive correlations between the shape of the spotted black bib, cell-mediated immunity and body condition have also been detected (L Pérez-Rodríguez and FR Mougeot, unpublished), whereas the size of black bands have been positively related to body condition in males and negatively to the heterophil:lymphocyte ratio in females (a physiological stress index), suggesting that they may act as a signals of quality in both sexes [31].

Experimental design

Seventy-seven partridges were obtained from eggs laid by 25 breeding pairs housed in outdoor cages at the Dehesa Galiana experimental facility (Ciudad Real, Spain) [26]. Cages were inspected daily, and the eggs removed, identified and immediately stored at 15°C, which arrested embryo development. Stored eggs were transferred to incubators every 15 days. Hatchlings from two successive incubation series were used (hatching dates: 8 and 23 June, 2008). Hatchlings were identified with plastic rings and kept in indoor aviaries with ad libitum food and water. Birds were randomly assigned to one of the four treatments (below) just before the development of their melanized plumage (i.e., about 20-days of age). Then, they were transferred to one of four different indoor aviaries (4×3×3 m; Ligth:Dark; 13 h∶11 h; ad libitum food and water). Diet was pelleted food (Perdix Vuelo, Superfeed, Madrid) and wheat (1∶1; see Text S1). Birds from the second incubation series were kept in four other aviaries under the same conditions. Birds received diquat (n = 22), α-MSH (n = 17) or both (n = 17), while a fourth group served as a control (n = 21). Treatments were balanced with regard to parents' identity, thus aiming to represent all treatments in each brood.

Just before the chicks were assigned to the treatments and placed in the aviaries (20 days of age), they were sampled for blood, weighed and their tarsus length measured with a caliper (“pre-treatment values”). The same was done at the end of the manipulation, i.e., 33 days later (“post-treatment values”). Blood was stored at 4°C and centrifuged within 5 h after extraction. Plasma and cell fractions were stored at −80°C. We introduced the hour of blood sampling as a covariate in models testing lipid peroxidation, triglycerides or cholesterol levels (see Statistical analyses below and Text S1).

Diquat treatment

Diquat dibromide is a molecule similar to paraquat that generates superoxide anion, one of the most abundant ROS, e.g., [32], [33]. The commercial product ‘Reglone’ (Syngenta, Madrid), which consisted of 20% w/v of diquat dibromide in water, was used. In our study, diquat was supplied in drinking water. The treatment with diquat or only water lasted 33 days, overlapping with the greater part of feather development. Each aviary contained a tank with treated water (Text S1). Therefore, each aviary contained a single drinking treatment (i.e., diquat plus water or only water).

The diquat dose (0.50 ml l⁻¹ in water) was established on the basis of a previous pilot study (Text S1). Taking into account water intake during that study, mean daily intake of diquat-treated birds was ≅ 7 µg of diquat. Body mass and tarsus length did not significantly differ between treatments neither before nor after the treatment [26]. Body mass gain and final body condition were not affected [26]. Changes in behavior and feces (diarrhea or hemorrhage) were daily inspected, but nothing was detected. No bird died during the pilot study or the subsequent manipulation, though some birds died before the color assessment (40 days after the end of the diquat treatment; below).

α-MSH treatment

α-MSH (Sigma, St. Louis, MO) was injected in the left pectoral muscle of each experimental bird (0.04 mgs of α-MSH in 2 ml of phosphate buffered saline; PBS). Control birds received 2 ml of PBS only. Injections were administered every two days during a 15 day period (i.e., 8 injections per bird). Each bird received a total amount of 0·32 mg of α-MSH. The total α-MSH dose used in this study is equivalent to that used by Höhn & Braun [34] (also Text S1). Both α-MSH- and PBS-injected birds were present in each aviary.

Molecular sexing

Blood cell pellet was used. DNA from sex chromosomes was amplified by PCR (primers 2550F and 2718R) [35].

Assessment of circulating carotenoid, cholesterol and triglycerides

Total plasma carotenoid levels were determined by spectrophotometry (Shimadzu UV-1603, Japan), using a standard curve of lutein (Sigma, St Louis, MO) (see Text S1).

Plasma levels of total cholesterol and triglycerides (two of the main lipoprotein components) were also assessed by spectrophotometry (A25, Biosystems SA, Barcelona). The cholesterol oxidase/peroxidase and glycerol phosphate oxidase/peroxidase methods were used to determine them, respectively (commercial kits; Biosystems SA, Barcelona, see Text S1). Lipoproteins serve as carotenoid carriers, and particularly, plasma cholesterol levels would indicate levels of those lipoproteins carrying carotenoids as they have been positively correlated with circulating carotenoid levels in birds, e.g., [5], [36]. Meanwhile, plasma triglycerides were assessed as a proxy of changes in intestinal absorption because these lipids are the main constituents of those lipoproteins (i.e., chylomicrons) in charge of lipid and carotenoid absorption from intestines to blood (about 93% of chylomicron mass) [37].

Color assessment of carotenoid-based traits

Digital photography (Olympus E-500 camera) was used after checking the relatively low repeatability of different spectrometers, probably due to the heterogeneous surface of partridge bare parts (see Text S1). Previous studies in the same species have shown that carotenoid-based color as assessed in the present study is associated with fitness-related variables [28]–[30], [38], [39]. We assume that technical limitations could have reduced the precision of the measure, but not its accuracy. Thus significant effects detected from our measurements would be revealed in spite of this limitation, but not due to methodological bias. See Text S1 for additional details and support for this technique.

Partridges were photographed at 93 days of life, when all the birds showed a fully developed adult phenotype. Three diquat-treated, two α-MSH-treated and one control bird died between the end of the treatment and this age (χ² = 3.12, d.f. = 3, P = 0.373). Thus, the color of seventy-one birds was finally assessed. Birds were held in the same posture and at a fixed distance from the camera by means of a repro lighting unit. To correct for subtle variability in the level of light received by the partridges, a standard red chip (Kodak) was placed close to the red traits of the bird (Text S1 for further details).

Hue values were obtained from mean RGB using the algorithm described in Foley & Van Dam [40]. A principal components analysis (PCA) was carried out to obtain a single variable from the three measures of redness. A single component explained 91.9% of variance. Eigenvalues were 0.930, 0.954, 0.874 for upper and lower mandible and eye ring, respectively. The three variables were positively correlated among them (all Pearson's r-values >0.82, all P's<0.001). As in the case of hue, high PC1 values denoted less redness. However, to facilitate the interpretation, the sign of the PC1 values was reversed. This new variable was termed as “red intensity”.

Assessment of melanin-based plumage

The expression of the melanin-based plumage was also analyzed from digital pictures and Adobe Photoshop at the same age. These pictures were different that those used for the redness assessment. The surfaces of black spotted bib and black and brown flank bands (pixels) were obtained (Text S1 and ref. [26]).

Statistical analyses

Generalized linear mixed models (PROC MIXED, SAS software) [41] were used to determine the experimental effects on red intensity and change in the level of circulating carotenoids and lipids (i.e., post-treatment minus pre-treatment value). These variables were dependent ones in single GLMMs, and diquat (presence vs. absence) treatment, α-MSH (presence vs. absence) treatment and sex were added as factors together with their interactions. The identity the pair that laid the egg and the aviary in which the chicks were reared were included as random factors. In the model testing red intensity, the hue of the red chip was added as a covariate (F_1,57.7 = 145.7, P<0.001). The pre-treatment value was included as a covariate in models testing blood parameters, e.g., [39]. To understand whether effects were mediated by body mass variability (i.e., potential differences in food intake or metabolism), body mass change was also added as a covariate. This covariate was the residual of the difference between post- and pre-treatment masses (dependent) corrected by the pre-treatment mass (independent). Lastly, the time of blood sampling was tested as a covariate to control for any influence of the last feeding event on lipid values (always p>0.20, and hence, removed).

Starting with the saturated model, a backward stepwise procedure was used, removing any term with P>0.05. Random factors were maintained in the models, though similar results were obtained when removed. Non-significant terms included in significant interactions were also maintained. The Satterthwaite correction was used to approximate the degrees of freedom. The distribution of residuals obtained from the models met the normality assumption. Only the results of the models obtained after the stepwise procedure are shown here. Full saturated models are reported in Text S1. Least squares means and slopes (± s.e.) were calculated from the models.

Effects of diquat and α-MSH on the expression of a carotenoid-based trait

Partridges exposed to diquat during development showed paler red traits than controls (Fig. 2; diquat treatment: F_1,61 = 5.63, P = 0.020; red reference chip F_1,57.7 = 145.7, P<0.001). The α-MSH-treatment, sex and interactions did not show significant effects, being removed from the final best fitted model (all P's>0.16; saturated models in Text S1).

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Figure 2. Redness of carotenoid-based ornaments of control partridges and partridges exposed to free radicals.

Red intensity is the inverse of a principal component summarizing variability in the hue of both mandibles and eye ring (methods). Least square means ± s.e. were obtained from the final model (results).

https://doi.org/10.1371/journal.pone.0019403.g002

Effects of diquat and α-MSH on circulating carotenoids and lipids

In the model analyzing variability in carotenoid levels, both diquat (F_1,38.1 = 4.73, P = 0.036) and α-MSH (F_1,59 = 6.03, P = 0.017) treatments had significant effects. Partridges exposed to diquat showed a weaker increase in carotenoid levels than control birds (0.59±0.46 and 1.81±0.47 µg ml⁻¹, respectively). In contrast, birds treated with α-MSH showed a greater carotenoid increase than controls (1.79±0.45 and 0.61±0.44 µg ml⁻¹, respectively). Body mass change (F_1,48.7 = 12.94, P = 0.001; slope: +0.041±0.011) and pre-treatment carotenoid level (F_1,26.8 = 69.2, P<0.001; slope: -0.776±0.093) remained in the model. For illustrative purposes, figure 3 represents the change in carotenoid levels separately for each experimental group. Nonetheless, the diquat x α-MSH interaction was not significant (P = 0.908).

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Figure 3. Change in the levels of several blood parameters during the experiment.

Circulating (a) carotenoids, (b) cholesterol and (c) triglycerides in partridges exposed to different treatments during development. Least square means ± s.e. were obtained from the final models (results).

https://doi.org/10.1371/journal.pone.0019403.g003

Partridges exposed to diquat also showed a weaker increase in cholesterol levels than controls (+168.2±63.2 and 315.3±59.4 µg ml⁻¹, respectively; F_1,46 = 4.75, P = 0.034; pre-treatment level: F_1,56.5 = 28.71, P<0.001, slope: −0.716±0.140). α-MSH, sex, body mass gain and interactions did not reveal any significant influence on cholesterol variability (all P's>0.19), and were removed from the model (also Fig. 3b). By contrast, the change in triglyceride levels was only explained by body mass change (F_1,50.9 = 4.10, P = 0.048, slope: 9.232±4.558) and pre-treatment value (F_1,60.7 = 57.9, P<0.001, slope: −0.925±0.122; other terms: P's>0.10; Fig. 3c).

Interestingly, if the change in cholesterol is added as a covariate to the final model for change in carotenoid levels (above; cholesterol change: F_1,56.4 = 5.06, P = 0.028, slope: +0.028±0.013), both diquat and α-MSH factors became non-significant (P = 0.157 and 0.141, respectively). However, the model for carotenoid levels was not affected by the change in triglyceride levels (always P>0.35).

Carotenoid- and melanin-based trait expressions interact under oxidative stress

We explored the influence of the variability in the expression of melanic traits on the expression of carotenoid-based traits. With this aim, we added the surface of black (eumelanic) spotted bib, black (eumelanic) and brown (pheomelanic) flank bands as covariates to the model for red color intensity (see above). Black and brown flank bands did not show any significant influence or interaction with any factor, and were removed from the model (all P's>0.06). However, the surface of the black spotted bib interacted with diquat-treatment (F_1,58.4 = 8.12, P = 0.006; Fig. 4). Red intensity was positively related to the area of the bib in diquat-treated birds (slope  =  +0.127±0.040, P = 0.004), and negatively related in birds not exposed to the pro-oxidant (slope = −0.110±0.062), though non-significantly different from zero (P = 0.17). If the bird with the largest bib is conservatively removed from the analyses (see Fig. 4), both the interaction and the relationship between redness and bib surface in diquat-treated birds remained significant (P = 0.015 and 0.022, respectively). Furthermore, if the analysis is restricted to birds that did not receive any treatment (n = 17), the negative relationship between bib surface and redness is significant (F _1,15 = 10.23, P = 0.006).

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Figure 4. Relationship between red intensity and size of the black spotted bib.

Partridges exposed to diquat (full dots and continuous line) and control birds (empty dots and spotted line). Red intensity values are residuals after controlling for red chip variability and random factors. Bib data are residuals after controlling for the effect of α-MSH-treatment and random factors (all P's<0.05). The lines were calculated from the model (see slopes in Results).

https://doi.org/10.1371/journal.pone.0019403.g004