Study sites

Deer mice were collected from 12 separate 10,000 m² trapping grids (100 traps distributed across 10, 100-m transects) located within a 65 km radius of Durango, CO. These sites were chosen because of high deer mouse densities and SNV prevalence. Trapping was conducted over a two-year period; early season trapping occurred in June 2009 and late season trapping occurred in July and August of 2010. These sampling periods were selected based on life history traits typical of wild deer mice, in which new SNV infections typically peak in April and May following the peak of reproductive activity (Kuenzi et al., 2005; Lehmer et al., 2010). Based on this assumption, wild deer mice are most likely to be in the acute phase of infection in June and then move into the chronic stage of infection by July. Although these methods do not guarantee the stage of infection of individual deer mice, they provide a high likelihood that our early and late samples contain a large number of mice in the appropriate stage of infection without extensive assays that were beyond the scope and budget of the present study.

Small mammal processing

After capture, small mammals were identified to species, weighed for body mass, and then reproductive condition was identified. Deer mice weighing under 14.0 g were considered juveniles (Lehmer et al., 2010) and were excluded from further processing. Juvenile deer mice receive maternal antibodies during gestation and lactation. This passive immunity persists for up to 4 weeks post weaning. Thus juvenile deer mice may test positive for SNV during this period without having an active SNV infection (Douglass et al., 2007). Approximately 0.3 ml of blood was collected from all adult deer mice via the retroorbital sinus using heparinized microcapillary tubes. A small subsample of blood (0.1 ml) was used to create a monolayer blood smear by placing a drop of blood onto a glass microscope slide and using another glass slide to feather the blood at a 45⁰ angle. Blood smears were allowed to dry and then were stored at 20°C for further analyses. The remaining blood was stored on dry ice in the field and later transferred to a −20°C freezer on the Fort Lewis College campus until further assays were run. After processing, rodents were released back to their capture sites. All procedures for trapping and handling small mammals were approved by the IACUC at Fort Lewis College and CDC guidelines for handling rodents potentially infected with SNV were followed.

Leukocyte profiles

Upon returning to the lab at Fort Lewis College, blood smears collected in the field were stained using the Wright 3-step protocol (Rodak et al., 2007). After staining, microscopes at 100x and 400x magnification were used to identify locations on slides where the monolayer smears were ideal for counting individual cells. Then, using oil immersion lenses at 1000x, leukocytes were systematically counted by moving horizontally and vertically across the entire surface of the slide. In this process all leukocytes encountered on a single slide were differentially classified as lymphocytes, eosinophils, basophils, neutrophils, or monocytes. Macrophages were neither encountered nor counted, as these leukocytes are typically differentiated from monocytes to macrophages as they cross the endothelium and are found only in tissues and not typically in whole blood (Chomarat et al., 2000).

SNV antibody detection

Using enzyme-linked immunosorbent assays (ELISA), SNV infection status of captured deer mice was determined. ELISA tests for the presence of SNV antibodies (IgG) in serum (Otteson et al., 1996). Because deer mice are chronically infected with SNV, they produce antibodies to SNV throughout life. Thus, presence of SNV antibodies in sera is a reliable proxy for determining SNV infection (Schountz et al., 2007; Easterbrook and Klein 2008; Clay et al., 2009). Prior to performing the ELISAs, deer mouse sera were heat inactivated in a laminar flow hood in the BSL-2 laboratory at Fort Lewis College. In this process, whole blood samples were placed in a 55°C water bath for 30 minutes, and then centrifuged to separate serum from whole blood. ELISAs were performed following the protocol described previously by Otteson et al. (1996) and Feldman et al. (1993). Briefly, 96 well plates were coated with recombinant SNV nucleocapsid antigen at 1:400 in phosphate buffered saline (PBS) and stored overnight at 4°C. After washing wells in PBS with 0.5% Tween-20 (PBS-T), heat inactivated serum samples were diluted 1:100 in PBS with 0.5% Tween-20 and 5% skim milk (milk diluent), plated in duplicate and then incubated for 60-120 minutes at 37°C. Goat anti-Peromyscus leucopus HRP secondary antibody was diluted to 1:1000 in milk diluent and incubated for 60 minutes at 37°C. After incubation, plates were washed three times in PBS-T and ABTS peroxidase substrate (Kirkegaard and Perry Laboratories) was added to the wells. Plates were incubated for 30 minutes at 37°C to develop the assay and then were read on a Tecan Infinite M200 plate reader. Deer mice were considered seropositive if their optical densities were > 3x negative control sera.

SNV prevalence

Over the course of two sampling seasons, we captured 97 unique deer mice (n=97). In 2009, we captured 51 deer mice, including 15 that were infected with SNV and 36 that were uninfected. In 2009, SNV prevalence on our study sites was 29.4% (Figure 1). In 2010, we captured 46 deer mice, including 9 that were infected with SNV and 37 that were uninfected. In 2010, SNV prevalence across our study sites was 19.6% (Figure 1).

Basophil levels

There were no differences in basophil levels between SNV infected and uninfected mice (infected mean = 0.019+ 0.010, uninfected mean = 0.029 + 0.006; F_1,93= 0.648, P = 0.423; Figure 2). However, basophil levels differed between seasons, with deer mice captured in the early season having greater numbers of basophils, compared to mice captured in the late season (2009 mean = 0.049 + 0.008, 2010 mean = 0.00 + 0.009; F_1,93 = 16.510, P < .000; Figure 3). There was no significant season x infection interaction (F_1,93=0.648, P =0.423).

Neutrophil levels

Neutrophil levels were influenced by SNV infection status, as infected deer mice had higher neutrophil counts compared to their uninfected counterparts (uninfected mean = 0.308 + 0.032, infected mean = 0.501 + 0.058; F_1,93 = 8.581, P = 0.004; Figure 2). Neutrophil levels were not influenced by seasons, as we found no differences in neutrophil counts between deer mice captured in early and late seasons (2009 mean = 0.374 + 0.042, 2010 mean = 0.435 + 0.051; F_1,93= 0.846, P = 0.360); however, there was a significant season x infection status interaction (F_1,93= 7.857, P =.006).

Eosinophil levels

There were no differences in eosinophil levels between SNV infected and uninfected mice (uninfected mean = 0.021 + 0.004, infected mean = 0.013 + 0.006; F_1,93=1.391, P = 0.241; Figure 2). However, eosinophil levels differed between seasons, with deer mice captured in the early season having greater eosinophil counts compared to deer mice captured in the late season (2009 mean = 0.034 + 0.005, 2010 mean = 0.001 + 0.006; F_1,93=21.395, P = 0.000; Figure 3). There was no significant season x infection interaction (F_1,93=1.391, P = 0.241).

Monocyte levels

Monocyte levels were influenced by SNV infection status, with uninfected deer mice having greater monocyte counts compared to their SNV-infected counterparts (uninfected mean = 0.428 + 0.030, infected mean = 0.256 + 0.055; F_1,93 = 7.515, P = 0.007; Figure 2). Monocyte levels also differed between seasons, with deer mice captured in the late season having higher monocyte counts compared to deer mice captured in the early season (2009 mean = 0.194 + 0.040, 2010 mean = 0.489 + 0.048; F_1,93 = 22.132, P = 0.000; Figure 3). There was a significant season x infection interaction (F_1,93=22.132, P < 0.001).

Lymphocyte levels

There were no differences in lymphocyte levels between SNV infected and uninfected mice (uninfected mean = 0.213 + 0.021, infected mean = 0.211 + 0.038; F_1,93 = 0.004, P = 0.947; Figure 2). However, lymphocyte counts differed seasonally, with deer mice captured in the early season having greater lymphocyte counts than deer mice captured in the late season (2009 mean = 0.349 + 0.027, 2010 mean = 0.075 + 0.033; F_1,93 = 40.460, P < .001; Figure 3). There was no significant season x infection interaction (F_1,93= 0.478, P = 0.491).

SNV prevalence

SNV prevalence in our study populations declined between the first and second years of the study; however, it is important to emphasize that, because the study populations in 2009 and 2010 were comprised of different individuals, these patterns are not reflective of an increased incidence of infection from early to late season. SNV prevalence is highly variable across both temporal and spatial scales and, because deer mice are relatively short lived, study populations that are repeatedly sampled over time often show dramatic fluctuations in SNV prevalence between sampling periods (Lehmer et al., 2008).

Seasonal trends

In our study, we looked to identify trends in seasonality and infection status. We observed similar seasonal patterns of basophil, eosinophil and lymphocyte profiles among deer mice, in that regardless of their SNV infection status, deer mice captured in the early season had greater numbers of these leukocytes compared to deer mice captured in the late season. Conversely, monocyte levels increased in the late season. Neutrophil levels were unchanged across seasons. These results are significant because they suggest that seasonal stressors may have a greater influence on immune system function than does infection with SNV. Because SNV does not cause acute illness in deer mice (Hjelle and Yates, 2001; Yee et al., 2003), it is possible that deer mice increase fitness by reducing their immune response to this non-lethal pathogen. Indeed, previous studies have described a similar “resistance – tolerance tradeoff” in other wild animals and have suggested that, by reducing the response to non-lethal pathogens, animals increase fitness, as tolerating a mild disease caused by non-lethal pathogens may be less physiologically demanding than the cost of mounting immunological resistance (Råberg et al., 2007; Boots, 2008). Furthermore, other researchers have proposed that offsetting fitness costs of SNV infection in this manner may have promoted the long and relatively stable co-evolutionary history that deer mice have with SNV (Schountz et al., 2007).

Seasonality has been cited as an important modulator of immune system function in wild mammals (Demas and Nelson, 1998a; Demas and Nelson, 1998b; Zhou et al., 2002). Previous lab studies focused on general immunity have shown that male deer mice exposed to shorter day lengths and lower ambient temperatures have increased leukocyte production compared to their counterparts exposed to longer day lengths and higher ambient temperatures (Demas and Nelson, 1998b). Similar studies in Syrian (Mesocricetus auratus) and Siberian (Phodopus sungorous) hamsters have shown that although photoperiod can affect leukocyte proliferation, activation of these leukocytes is not dependent on photoperiod (Zhou et al., 2002). Because our study focused on the relative abundance of leukocytes in finite blood samples, rather than on total leukocyte counts, we cannot make predictions about overall immunocompetence of deer mice in our study. However, our study design allows us to infer priority in leukocyte production across seasons. Our study took place between the months of June and August, when the photoperiod ranged from 14h 42m in mid-June to 13h and 35m in mid-August, spanning a little over an hour photoperiod difference between the early and late seasons (Weather Underground, Inc., 2011). While this difference in photoperiod may seem small, it represents a shift between two seasons (reproductive and non-reproductive) in the short life (> 6 months) of a deer mouse. In our study, longer photoperiods were associated with deer mice having elevated basophil, lymphocyte, and eosinophil levels, which are generally upregulated in response to allergens, viral infections and parasitic infections, respectively (Tizard, 1984; Gleich and Adolphson, 1986). In contrast, deer mice captured during seasons with shorter photoperiods had substantially elevated monocyte levels, comprising over 48% of the total leucocytes counted. Wild deer mice cope with a number of biotic and abiotic stressors, including shifts in forage quality and availability, as well as energetic costs of thermoregulation, evading predation, exposure to other pathogens and reproduction. Each of these factors imposes demands on the energy budgets of small mammals, which in turn affects their immunocompetence (Klein et al., 2000; Lehmer et al., 2007). Thus, deer mice may balance these energetic demands by allocating resources to immune system function differentially across seasons. Collectively, our results seem to support the notion that immune stressors faced by wild deer mice shift from early to late season, and these differences are reflected by differential leukocyte production that occurs across seasons.

SNV infection status trends

Although we observed no difference in basophil, eosinophil and lymphocyte levels between SNV-infected and uninfected mice, SNV infection did appear to influence monocyte and neutrophil production. Whereas monocyte levels were greater in uninfected deer mice, neutrophil production was greater in SNV-infected mice. These results indicate that the inflammatory immune response of wild deer mice is elevated in response to SNV, as neutrophils initiate a cascade of pro-inflammatory cytokine production, including production of TNF-α. These findings are potentially significant in that they differ from those reported for captive deer mice infected with SNV. Previous lab-based studies have shown that chronically infected reservoirs of hantaviruses suppress inflammatory immune pathways and inflammatory cytokine production (Schountz et al., 2007; Easterbrook and Klein 2008). In contrast, humans have substantially elevated pro-inflammatory immune responses to SNV, which is often fatal. Specifically, humans infected with SNV often experience marked increases in TNF-α production, which is likely the cause of increased permeability of endothelial capillaries that ultimately results in severe pulmonary edema, the hallmark of HPS (Yates et al., 2002; Borges et al., 2008; Easterbrook and Klein, 2008; Mori et al., 1999). Although measuring cytokine production was beyond the scope of the present study, our results highlight potential differences between the immune responses of wild and lab-bred deer mice to SNV, as well as some potential similarities in the immune response to SNV between wild deer mice and humans. Future studies should more closely evaluate patterns of cytokine production in wild deer mice infected with SNV.

We acknowledge that our study has a number of limitations that are inherent in studying infection in wild mammal populations, including, for example, an inability to pinpoint date of infection and to obtain localized versus peripheral blood samples. However, because wild deer mice are responsible for transmission of SNV to humans, field-based studies provide valuable insight about factors that regulate SNV transmission in the natural environment. Thus, despite these limitations, future studies should continue to examine the immune response of wild deer mice to SNV infection.