Study area

The study area comprised 23 locations in the Rhône department (i.e. administrative spatial unit) of France, which encompasses the city of Lyon and 14 farms within 30 km of our laboratory (45° 47′ 30·93′ N; 4° 42′ 30·28′ E). This area contains a range of urbanization levels. Farms were requested to participate based on their inclusion in previous surveys, and all agreed. The dwellings and public areas were selected based on high rat concentrations reported by the Hygiene Service of Lyon.

Most farms were medium to large size (i.e. > 100 animals) with mixed livestock. The nine urban trapping locations were distributed in dwelling areas, public gardens, waste disposal areas, and an industrial area in the city centre and suburbs.

Sampling

The survey was subdivided into 6-month periods: (1) September 2010 to February 2011 and (2) October 2011 to March 2012. To account for possible seasonal variation in the pathogen prevalence, the two periods encompassed the same season. The sampling size (n≈90) was calculated using a 95% confidence level, a relative accuracy of 50%, and an expected prevalence of 10–30% [Reference Thurdfield16]. To account for possible variation in the pathogen prevalence among different urbanization levels, the same sample size was used in areas of low and high population density. During the two periods, 178 free-living Norway rats were trapped in areas of low (n = 94) and high (n = 84) population density.

Most rats were captured with small (28 cm × 9 cm × 9 cm) or large (50 cm × 15 cm × 15 cm) single-catch rat traps. The captured rats were transported to the laboratory and immediately anaesthetized using isoflurane. A blood sample was obtained by cardiac puncture. Subsequently, the rats were sacrificed by cervical dislocation. The rats that succumbed to capture were frozen at −20°C and thawed on the day of dissection. Data were recorded on weight, size, sex, sexual maturity (i.e. the presence of seminal vesicles in males and a developed uterus in females) and pregnancy. Lung and liver lobe fragments weighing between 50 and 100 mg were collected, and the kidney was removed. The heart was incorporated in an antibiotic solution with 1·2 × 10⁻⁵ g/ml amoxicillin (Amoxicilline Panpharma, France), 120 UI/ml penicillin and 120 μg/ml streptomycin (Pen-Strep Liq 10 000, Gibco, USA). Faecal samples were collected from the rectum, and all tissue and faecal samples were stored at −80°C immediately following collection.

The authors assert that all procedures contributing to this work comply with the ethical standards of the relevant national and institutional guides on the care and use of laboratory animals (agreement no. 69-020931).

Screening protocols

L. interrogans colonization of the kidney was assessed via culture [Reference Zuerner17] and a pathogen-specific L. interrogans TaqMan real-time polymerase chain reaction (PCR) kit (TaqVet PathoLept kit, LSI, France); additionally, the rpoB gene was targeted. Lung tissues were screened for hantavirus using a nested pan-hantavirus reverse transcription (RT)–PCR selective for partial polymerase large segment (L) gene sequences, subsequent molecular typing was performed to determine the hantavirus species as previously described [Reference Dupinay18]. The HEV viral load in the liver and faeces was analysed using TaqMan real-time PCR reagents specific to rat-strain HEV and genotypes 1–4 [Reference Widèn19]. Sera extracted from blood-soaked blotters were tested for T. gondii antibodies using a modified agglutination test (MAT) that detects T. gondii-specific IgG antibodies [Reference Dubey and Desmonts20]. The hearts of animals with a positive agglutination (starting dilution 1:6) were bioassayed in mice to isolate viable T. gondii [Reference Villena21].

Prevalence calculation

L. interrogans, SEOV, and HEV were screened based detecting pathogen nucleic acid sequences or the microorganism itself; rats testing positive were considered to be infected and potential shedders of the pathogens. The rats with MAT-positive results were considered to be exposed because the presence of antibodies against the pathogen could result from previous or current contact with the pathogen. The prevalence of infected or exposed rats was defined as the proportion of rats with any positive test results. The apparent prevalence was restricted to the population sampled since and the administrative unit of the Rhône department

Variables

Two categories of explanatory covariates were considered: rat-related and socioeconomic covariates. Rat survival during the trapping was also considered, as death and freeze–thaw cycles before dissection could alter the sample quality and underestimate the prevalence.

The rat data included the species (determined by external morphology and macroscopic observations), sex, weight, size, and approximate age, based on sexual maturity and pregnancy. A body mass metric was constructed from the residuals that resulted from the regression of weight on size [Reference Sokal and Rohlf22]. The capture success, a proxy of the population size, was accurately defined in five sites by

$${\rm capture}\;{\rm success} = \displaystyle{{n_i} \over {t_i \times d_i}}, $$

where n _i is the number of rats captured, t _i the number of traps set and d _i the number of days of trapping at the site i.

The extent and features of urbanization were characterized using the socioeconomic data. Eleven candidate variables were extracted from the 2009 national census data provided by the Institut National de la Statistique et des Etudes Economiques. Remotely sensed data were obtained at the smallest geographical unit, which is the Ilot Regroupé pour l'Information Statistique (IRIS). Each IRIS contains 2000 inhabitants. The socioeconomic variables are displayed in Table 1.

Table 1. Description of socioeconomic covariates

Spatial analysis

The location and number of rats in each trapping area that tested positive and negative were mapped using ArcGIS version 9.3 (ESRI, USA). Spatial clusters of high and low pathogen prevalence were identified using the Getis-Ord Gi* statistic. The local sum for features and the feature's neighbours were compared proportionally to the sum of all features. When the local sum was statistically significantly different from the expectation, the region was denoted as having low or high prevalence.

To identify the potential socioeconomic proxies of RBZ, the candidate variables from the census data sets were extracted from the IRIS units with trapping locations. An approach using various boundaries for the quadrats when extracting data was implemented to verify the effects of different spatial scales on the risk factors [Reference Diez-Roux23]. The socioeconomic data were extracted using four quadrat sizes: 100 m × 100 m, 200 m × 200 m, 400 m × 400 m, and 800 m × 800 m. The socioeconomic metrics for each quadrat were calculated by weighting the remotely sensed data by the percentage of the IRIS surface that was included in the quadrat. For each spatial level of analysis, a new data set was obtained by spatial query using the software R project version 3.0.1 (R Development Core Team, Austria) and ArcGIS version 9.3 (ESRI, Redland, CA, USA).

Statistical analysis

To identify the characteristics associated with each pathogen's carriage status, distributions of the explanatory variables were examined within the samples testing positive and negative. χ ² tests and Wilcoxon tests were used, as appropriate, and an alpha level of 0·05 was used to reject the null hypothesis. For each pathogen, the potential effect of the population size on the number of infected rats in the trapping sites was assessed by testing the Pearson correlation between the capture success and the related number of infected rats. An α-level of 0·05 was used to reject the absence of correlation. The result obtained determined whether the capture success had to be considered in the models.

Statistical modelling was performed to evaluate the use of rat-related criteria and socioeconomic indices as predictors of exposure or infection in rats. All remotely sensed data were transformed to be normally distributed when they were incorporated into the models, and missing data were not considered. Simple logistic regression (SLR) was used to examine the relationship between each pathogen's prevalence and the explanatory variables. Covariates that were significantly associated with pathogen infection or exposure at an α-level of 0·10 were considered for further analysis. To select independent variables, rat-related covariates were tested for multicollinearity using Spearman's rank correlation (ρ > 0·7) with the Hmisc package in R, whereas socioeconomic covariates were described with a principal component analysis (PCA) using the FactoMineR package in R. From the PCA result, one variable per main axis was chosen based on the comprehensiveness of the data. Selected covariates were incorporated into multivariate models. The variation inflation factors were calculated with the car package in R to verify a low effect of potential collinearity (<5).

When the effect of rat death during capture was significantly associated with the infection status in SLRs, the data set was adjusted to account for a possible sample alteration effect.

For each pathogen, two multivariate logistic regression models were implemented. The selected covariates were incorporated into a generalized linear model (GLM) as fixed effects. The final GLM was selected using Aikake's Information Criterion (AIC) to balance model fit and parsimony. Then, the adjusted effects of the variables included in the final GLM were estimated with a generalized linear mixed model (GLMM) to control for the random effect of trapping locations and to account for the potential effects of clustering.

The remotely sensed data extracted from the quadrats were considered for each socioeconomic variable included in the final GLMs. A new set of models was created to account for the possible influence of changing spatial scales on the adjusted effects.