Study area

We carried out faeces sampling in a site covering 2,500 ha and situated in the Palatinate Forest in the federal state of Rhineland-Palatinate, southwestern Germany (49°12‘N, 7°45‘E). Elevation ranged between 210 m and 609 m a.s.l. The predominant native plant community was beech Fagus sylvatica forest (Luzulo-Fagetum). The area was covered with forest by approximately 90% (i.e. 44% beech, 26% pine Pinus sp., 10% Norwegian spruce Picea abies, 12% Sessile oak Quercus petraea and 8% common oak Q. robur; Reis 2006). Several small settlements with surrounding open areas occurred in the periphery of the study area. The annual average temperature is 8-9°C (Weiß 1993) and the annual precipitation approximates 600-1,000 mm. Artificial feeding of wild boar was forbidden in the federal state, but baiting was legal for hunting at registered sites when ≤ 1 litre of maize was given/site and day.

The annual harvest of wild boar in the state-managed hunting areas between 1999 and 2009 averaged 2.4 individuals/km² (range: 1.14-5.23 individuals/km² and year; Reis 2006, G. Scheffler, Forestry Office of Hinterweidenthal, pers. comm.). The hunting bag in the year before our faeces sampling was comparably low (1.8 wild boar/km²), whereas it was rather high in the year of our study (3.5 wild boar/km²). Hunting was carried out both via single hunts all year round and via drive hunts. Drive hunts were carried out in segments of 3-5 km² between mid-October and the end of January every two to three weeks, covering the whole study area during one season.

Field sampling

We carried out sampling during 14-31 January 2008. No hunts were carried out within our sampling period. We collected wild boar faeces along 16 transects of approximately 6-8 km length each (Fig. 1). Transects were installed parallel to each other in a north-south orientation (overall length: 104 km). Trails, small roads or streams were crossed, if necessary, but we avoided conducting transects along trails or roads to prevent potential bias of sampling results. We chose the parallel north-south transect design with the aim to cover the study area as representatively as possible by including all occurring habitat types and altitudinal levels. We aimed at maximising the collection of fresh faeces by walking the same transect routes in every repetition. We marked transect routes using spray paint on trees. The transect width, which could be effectively searched for wild boar faeces by a walking person, was approximately 3 m. We searched each transect for faeces every 48 hours and thus a total of six times during 12 days of one trial. The transects were walked by eight persons altogether, each covering 1 transect/day.

To increase our faeces finding rate, we applied a simplified form of adaptive cluster sampling (Thompson 1991). Every time we found a faeces sample, the field worker paused walking the transect and searched the area surrounding the sample in a radius of approximately 5-6 m. If further wild boar faeces were found within this radius, the search was extended in the respective direction. After having completed a cluster, the field worker continued walking the regular transect route. Thereby, we aimed at accounting for the fact that wild boar, at least females and their offspring, regularly occur in groups, and thus often faeces of more than one individual can be found in close proximity (Briedermann 2008). The maximum distance from the main transect route for cluster sampling was approximately 30 m.

We collected whole faeces using inverted freezer bags, which were then reversed and closed. Samples were stored frozen (at −19°C) in the sealed freezer bags for 6-8 months until analysis.

DNA extraction and genotyping

We extracted genomic DNA from all faecal samples using the NucleoSpin soil kit (Macherey-Nagel, Düren, Germany) following the manufacturer's instructions. For extraction, we scraped off material from the surface of the faecal pellets with a fresh scalpel for every sample. We established a qRTPCR on transgelin as a single copy gene (Acc. No. XM_003357308, Sus scrofa smooth muscle protein 22-alpha, mRNA) and used PRIMER3 software (Rozen & Skaletsky 2000) to design a suitable primer pair. The oligonucleotide sequences of this primer pair were as follows: 5‘-TAT CCT GAC GGC TCC AAA CCC-3‘ (forward, TAGLN1sus) and 5‘-CAG TCT TGG TGA CGC CAT AGT CC-3‘ (reverse, TAGLN2sus). We performed qRTPCR reactions in a total reaction volume of 15 μl containing 9 μl LC480 Sybrgreen Mix (Roche, Mannheim, Germany), 0.03 μl of each primer (100 μM), 2.94 μl H₂O and 3 μl DNA (diluted 1:5). We used a LightCycler®480 II (Roche) under the following conditions for qRTPCR: initial denaturation for 10 minutes at 95°C, followed by 45 amplification cycles with 15 seconds of 95°, 25 seconds of 59° and 35 seconds at 72°. We carried out the final melting curve assessment during a temperature increase from 60 to 95°C. We calibrated the absolute DNA quantification using a dilution series of a tissue derived DNA standard as described in Hausknecht et al. (2009) and defined a cycle threshold of 0.01 ng (C_t = 32) target DNA to exclude low quality samples from further analysis.

We used all samples containing a sufficient amount of target DNA according to the qRTPCR for further analyses. For microsatellite analysis, we used GeneAmp®PCR System 9700 Cycler (Applied Biosystems, Darmstadt, Germany) at the following PCR conditions: initial denaturation at 95°C for 15 minutes followed by 45 cycles of 30 seconds at 94°C, 30 seconds of 57°C and 60 seconds at 72°C, and a terminal elongation step at 60°C for 30 minutes. We performed amplification reactions in triplicates, each in a total volume of 12 μl using the Qiagen Multiplex PCR kit (Qiagen, Hilden, Germany). We used the primers at concentrations of 0.075 μM to 0.3 μM. We ran amplification products on an ABI3730 Sequencer using the ABI GS500LIZ size ladder, and we analysed them using the software GeneMapper v 3.7 to determine allele lengths (Applied Biosystems, Darmstadt, Germany). We carried out individual identification based on six microsatellite loci: TNFB, CGA, S0005 (Lowden et al. 2002), SW2496, SW2021 and SW742 (Rohrer et al. 1994, Kolodziej et al. 2011; see Table 2). For sex determination, we amplified the PigSRY gene (Kawarasaki et al. 1995). We combined the selected markers and co-amplified markers in one multiplex PCR. The markers S005 and SW2496 were amplified together in one additional run for every sample.

We calculated the probability of identity (P_ID) and the P_ID between siblings (P_IDsibs) using GIMLET (Valière 2002) to test if the combination of loci was sufficient to discriminate between individuals for the purpose of population estimation in our studied population (Waits et al. 2001). All samples were typed three times, and we determined a consensus genotype from the three results by applying the following rules: a sample was assigned a heterozygote when both alleles were observed at least twice, and to be classified as homozygous, the allele had to be observed three times. All samples showing ambiguous results after the first three repeats were typed another three times. We discarded samples which failed to amplify for two or more loci or did not show an unambiguous genotype after six (for markers S0005 and SW2496 eight) repeats from further analysis. We analysed genotyping results using GENECAP (Wilberg & Dreher 2004) and calculated genotyping error rates (allelic dropout ADO and false allele FA) according to Broquet & Petit (2006).

Using these error rates, we calculated global error rates (E_T and E_1or2) and final error rates (E_T-E_1or2) as developed in Puechmaille & Petit (2007) using an R script provided by S.J. Puechmaille (unpubl. report).

Population size estimation

We used maximum likelihood mixture models for closed captures with heterogeneity (Pledger 2000) implemented in program MARK (White & Burnham 1999) to estimate population size. We defined a set of plausible candidate models with varying assumptions concerning capture probability (p), choosing nomenclature according to Otis et al. (1978) for simplicity: M_Null as the most parsimonious model with capture probablity being constant over time and among individuals, M_h (heterogeneity; a mixture model incorporating two groups of animals with differing p), M_t (p varying over time) and M_th (heterogeneity and p varying over time). For each of these four basic models, we considered two different cases: ‘basic model only’ and ‘basic model including sex’ (two attribute groups).

Furthermore, we constructed capture histories for population estimation in two ways: For the first, we included only detections of the same individuals on different sampling days as ‘recaptures’, i.e. multiple captures during one sampling day were pooled to a single capture for each of the six sampling events. In the following, we will refer to this approach as ‘detections on different days only’, or DDO. For the second, we included all possible recaptures, i.e. plus multiple detections of individuals on the same day (see also Miller et al. 2005, Ruell et al. 2009), and shifted one of these detections back in time one day to fit in the capture history (the maximum number of detections recorded for the same individual per day was two). We will refer to the second approach as ‘maximum number of detections’ or MND.

For each of the two approaches, we calculated population size using all eight models. Additionally, we calculated model averages (i.e. weighted average over all models according to their model weight and thus according to their GOF; Burnham & Anderson 2002). As in program MARK, confidence intervals (CI) for model averages do not account for the minimum number of wild boar observed in the sampling area, we calculated CI using the unconditional SE and the equations reported in Rexstadt & Burnham (1991:19). For management reasons, we additionally aimed at obtaining CI for the total population (male + female). The population sizes and CI are estimated separately for both sexes, when sex is included as a grouping variable as it is the case in our analysis. Therefore, we calculated the sum of a random number of the female and male probability distribution, iterated this 10.000 times and calculated mean (total population size) and standard error from the resulting distribution. We used mean and standard error to calculate 95% CI based on the corresponding (Rexstadt & Burnham 1991) equations.

In addition to the closed capture mixture model estimates, we calculated population estimates using a single sampling session Bayesian model (Gazey & Staley 1986, Petit & Valière 2006), which is especially suitable for non-invasive data because it can make full use of all sampling information in the data set. To examine the assumption of capture homogeneity, we carried out a test in which we simulated the sampling process under the assumption of homogeneity and that the expected number of captures is compared with the observed number of captures/individual (Puechmaille & Petit 2007). We performed the Bayesian estimate and the test using the R package (Ihaka & Gentleman 1996) and a script provided by E. Petit (pers. comm.).

Population density

For the purpose of comparison with other wild boar populations and other studies as well as for comparison with the hunting bag per km² in the study area, we calculated population densities. Due to the short time span of sampling and because there were no drive hunts and most probably no births during each sampling trial, we consider the assumption of demographic closure as met in our study (Otis et al. 1978). However, there was no possibility to obtain topographic boundaries for the study area; thus, it can not be considered as geographically closed. The small sample size prevented us from applying models for open populations for population estimation (Luikart et al. 2010). Therefore, we added a buffer zone around the transect grid to calculate the effectively sampled area (ESA). We then used the ESA for calculating population density. We determined the width of the buffer using VHF- and GPS-telemetry data collected from wild boar tracked in our study area (C. Ebert, unpubl. data). We chose the radius of a mean monthly home range (95% Minimum Convex Polygon) as a buffer for calculating the ESA (see e.g. Tioli et al. 2009). This resulted, with a mean monthly home-range radius of 1,000 m, in an ESA of 52 km².

Hunting efficiency

To evaluate the efficiency of the hunting regime in our study area, we calculated an estimate of the reproductive output for comparison to the hunting bags for the given year. To calculate reproductive output, we assumed a population growth rate of 250% per year which was derived from combined data on wild boar reproduction in our study area and in a similar forested habitat also situated in southwestern Germany (Gethöffer et al. 2007). As a basis for the calculation of reproductive output, we used the Bayesian population estimate for each study year, because it seemed to be the most robust and conservative approach with our data.

Field sampling and genotyping

During the 2008 sampling period, we collected 515 wild boar faeces (i.e. 0.23 samples/km of transect searched). Based on the qRTPCR-results, 270 samples (i.e. 52%) contained a sufficient amount of target DNA and were used for further analysis. Of these, 244 (90%) yielded a complete 7-locus consensus genotype. From these, we identified 149 individuals, 66 males and 83 females, equivalent to a sex ratio of 1:1.26 (Table 1). P_ID and P_IDsibs were 4.73 × 10⁻⁸ and 0.00134, respectively. Of the 149 individuals, 53 (36%) were detected more than once, and the number of detections/individual ranged from one to six.

Mean ADO rate per locus was between 0.037 and 0.071 (Table 2). The observed FA rates ranged from 0 to 0.004. The multilocus error rate (E_T) estimated using equation 6 in Puechmaille & Petit (2007) was 0.0384733. This represents the probability of a genotype containing at least one error. The probability of a genotype containing exactly one or two errors (E_1or2) was 0.0384676. Consequently, the probability of a genotype containing more than two errors is 0.000005747. Because genotypes potentially containing one or two errors can be found in most cases by carefully rechecking all genotypes differing only at one (1-MM) or 2 (2-MM) loci, the latter represents an approximation of the residual error probability. According to these estimates and the number of analysed samples, the expected number of genotypes containing one or more errors (under the assumption that consensus genotypes are correct) is 9.4 with a 99.9% chance of representing exactly one or two errors.

Population size estimation

When comparing the maximum likelihood estimates for the DDO approach, the most supported model is M_h, which received 35% of the total model weight, followed by models M_Null and M_b with model weights of 20 and 15%, respectively (Table 3). The other models were considerably less supported and had AIC_c of > 2. None of the models with separated parameters for each sex received considerable support. The model averaged population estimate in the case of DDO indicates a total population size of 261 (207-366) wild boar. For the MND approach, only the M_h and M_hsex models received considerable support (sharing 99.5% of the model weight of which 77.3% are attibuted to M_h) with all other models showing AIC_c of > 10. The model-averaged population estimate indicates a total population size of 235 (199-297) wild boar. For both the DDO and MND approach, the male population estimates are less accurate than those for the females (see Table 3).

The Bayesian approach yielded an estimated population size of 236 (151-403) wild boar. In the simulation test, at least one of the observed values was outside the 95% CI of the expected values, thus indicating capture heterogeneity (Appendix I, Fig. 1).

Population density and hunting efficiency

Population density calculated using the model averaged population estimates is 5.0 wild boar/km² (95% CI: 4.0-7.0) for the DDO approach and 4.5 wild boar/km² (95% CI: 3.8-5.7) for the MND approach (see Table 3). Using the Bayesian population estimate yielded a population density of 4.5 (95% CI: 2.9-7.8) wild boar.

The reproductive output estimated from the Bayesian population density estimates is 6.8 (95% CI: 4.4-11.6) wild boar/km², leading to a total spring population size of 11.3 (95% CI: 7.2-19.3) wild boar/km² (Fig. 2). The 2008/2009 harvest density of 3.5 wild boar/km² thus corresponds to 31% (95% CI: 48-18%) of the estimated summer population (i.e. population including output) and to 51% (95% CI: 80-30%) of the reproductive output (Fig. 3).

Management implications

We selected a conservative estimate of population density as well as a moderate reproduction rate (Bieber & Ruf 2005) to calculate reproductive output for comparing to the hunting bag in the study area. However, the number of harvested wild boar corresponded to only 31% of the estimated summer population size, and even when taking into account the lower confidence interval of the population estimate, the harvest rate is approximately 48% of the estimated summer population size. Thus, the current hunting regime in our study area does not seem to be sufficient for regulating the wild boar population, even though the state agencies in charge aim to reduce the population (G. Scheffler, Forestry Office of Hinterweidenthal, pers. comm.). Since 1999, the mean hunting bag in the study area has increased almost threefold. To anticipate a further increase in population size, and even more to reduce the wild boar numbers, either the hunting regime will have to be changed (e.g. hunt more females of all age classes, especially piglets; Gethöffer et al. 2007, Toigo et al. 2008) or other regulatory mechanisms will have to be established (e.g. contraceptives; Massei et al. 2008). Artificial feeding is most probably no important factor in our study area, as feeding is forbidden and baiting only allowed in very restricted amounts, but may be so in other areas. In this case, the first thing to counteract population increase is to stop feeding wild boar. The data which we present here certainly are only a ‘snapshot’ of the wild boar population size in the study area and thus the management implications are of rather exemplary character. In order to effectively draw conclusions for management, a population should be monitored over several consecutive years.

Our study area is only one example; it is a known problem in many regions that hunting is not efficient in regulating wild boar populations. Nevertheless, until now there has been no measure for the extent to which hunting can achieve a reduction of a population or how far it is away from achieving a sufficient reduction. The method presented in our paper represents a tool to quantify the success of hunting or other management measures and thus serve as a calibration for wild boar management.

However, in order to allow more reliable and precise population estimates and thus more fine-grained conclusions for management, the sampling probability will have to be increased. Further studies should focus on the development of sampling strategies that allow a better representation of the sampled population in terms of number of unambiguously identified genotypes. Thus, faeces sampling efficiency and the combination with other strategies (e.g. genetic sampling of the hunting bag) are relevant parameters for research, but also the improvement of genotyping success.