Comparative analysis of humoral immune responses and pathologies of BALB/c and C57BL/6 wildtype mice experimentally infected with a highly virulent Rodentibacter pneumotropicus (Pasteurella pneumotropica) strain

Background

Mice are a natural host for Rodentibacter (R.) pneumotropicus. Despite specific monitoring, it is still one of the most important infectious agents in laboratory animals. The objective of this study was to determine the virulence of a prevalent pathotype of R. pneumotropicus and characterize the host response in a new animal model.

Results

Intranasal infection of C57BL/6 and BALB/c mice with a R. pneumotropicus strain (JF4Ni) bearing the genes of the three known repeats in toxin (RTX) toxins resulted in an unprecedented high mortality and morbidity above 50 and 80%, respectively. Morbidity was associated with severe weight loss as well as conjunctivitis and dyspnea. A main pathology was a catarrhal purulent to necrotic bronchopneumonia. Specific immune globuline (Ig) A was detected in tracheonasal lavages of most surviving mice which were still colonized by R. pneumotropicus. Furthermore, all surviving animals showed a distinct production of IgG antibodies. To differentiate T-helper cell (Th) 1 and Th2 immune responses we used subclasses of IgGs as indicators. Mean ratios of IgG2b to IgG1 were below 0.8 in sera drawn from both mice strains prior infection and from BALB/c mice post infection. In contrast, C57BL/6 mice had a mean IgG2b/IgG1 ratio of 1.6 post infection indicating a Th1 immune response in C57BL/6 versus a Th2 response in BALB/c mice associated with a tenfold higher bacterial load in the lung. In accordance with a Th1 response high antigen-specific IgG2c titers were detected in the majority of surviving C57BL/6 mice.

Conclusions

R. pneumotropicus JF4Ni is a highly virulent strain causing severe pneumonia and septicemia after intranasal infection of C57BL/6 and BALB/c mice. Persisting infections in the two mice strains are associated with Th1 and Th2 immune responses, respectively, and differences in the bacterial burden of the lung. The described model is ideally suited for future vaccination studies using the natural host.

Pasteurella (P.) pneumotropica was thought to be a species occurring mainly in two different biotypes: Jawetz and Heyl [1, 2]. However, P. pneumotropica was very recently reclassified and these two biotypes belong now to two different species, namely Rodentibacter (R.) pneumotropicus and R. heylii, respectively [3]. The differentiation of the two biotypes is based on the phenotype of the colony colour (grey and yellow, respectively), but polymerase chain reaction (PCR)-based differentiation is also possible [4,5,6]. In a recent study [7] differences in distribution of virulence factors between the two biotypes are described. Three different repeats-in-toxin (RTX) toxins, designated PnxI, PnxII and PnxIII, have been identified in P. pneumotropica. Whilst PnxI and PnxII are secreted and act as haemolysins or cytotoxins [8], PnxIII is associated with the bacterial membrane. Specifically, PnxIII interacts with the extracellular matrix [9, 10] but can also induce host cell cytotoxicity [9, 10]. Therefore, these RTX toxins are considered as important virulence factors [9].

P. pneumotropica is among the most important pathogens in laboratory animal populations with a reported prevalence of 4 to 13% in Europe and North America, respectively [11]. It is described as an opportunistic pathogen with low virulence in immunocompetent mice [2] but clinical signs were recorded in immunodeficient and –suppressed mice or in co-infections with Mycoplasma pulmonis [12] or Pneumocystis carinii [13]. Infected animals are generally unsuitable for scientific research due to suppurative to necrotizing lesions in various organs [14] and modulation of the immune response [15]. The Federation of Laboratory Animal Science Association (FELASA) lists P. pneumotropica as an important pathogen in mice, rats and hamsters and recommends the examination every 3 months [16]. Various monitoring methods are described including PCR [4, 5, 17] and indirect enzyme-linked immunosorbent assays (ELISAs) [18,19,20].

It is common practice to use soiled bedding sentinels for health monitoring of laboratory animals. Nevertheless, studies revealed a limited survival of P. pneumotropica in the environment [21, 22] and the failure of detecting P. pneumotropica infections by bedding sentinels [23].

In this study, we evaluated the pathologies and immune responses induced by experimental infection of BALB/c and C57BL/6 mice with a R. pneumotropicus pathotype emerging in German laboratory animal facilities. The new intranasal model leading to severe pneumonia, septicaemia but also to persisting infections is important for future studies on virulence and protection.

Distribution of pnxIA, pnxIIA and pnxIIIA in R. pneumotropicus and R. heylii

Different genes encoding RTX-toxins have been identified in P. pneumotropica, namely pnxIA, pnxIIA and pnxIIIA. By PCRs targeting these pnx genes, we investigated recently collected 27 R. pneumotropicus and 26 R. heylii strains. This profiling revealed that the distribution of pnxIA, pnxIIA and pnxIIIA differs substantially between the two species (Table 1). In 46% of the R. heylii strains only pnxI was detected. The gene pnxII was not found at all in this species. Twelve percent of the R. heylii strains carried both pnxIII and pnxI, whereas 43% were PCR negative for all RTX genes. In contrast, all three RTX genes were found in 74% of the R. pneumotropicus strains. Only 7% of the R. pneumotropicus strains did not carry any of the pnx genes. For further investigation, a recently isolated pnxIA+, pnxIIA+ and pnxIIIA+ R. pneumotropicus strain (JF4Ni) was chosen, because of its prevalent genotype identified by the screening of strains collected in Germany.

Morbidity, mortality and histopathology of experimentally infected animals and sentinels

Intranasal infection with 10⁸ CFU R. pneumotropicus JF4Ni resulted in 100% (16/16) morbidity in BALB/c and 87.5% (14/16) morbidity in C57BL/6 mice within one day. Fifty-six percent (9/16) of BALB/c died or had to be euthanized within 2–4 days after infection and 50% (8/16) of C57BL/6 within 3–6 days after infection (Fig. 1a). Diseased mice showed unspecific signs such as ruffled coat, bended back, heavy weight loss (Fig. 1b), dehydration as well as specific signs such as dyspnoea, conjunctivitis and mild incoordination in two cases. Significant differences in mortality and morbidity were only recorded between infection animals and controls, but not between the two mouse strains. All early deceased mice showed multifocal moderate to severe catarrhal-purulent bronchopneumonia, in some cases with necrosis (Table 2 and Fig. 1c). These pathologies were not recorded in mice which survived the experimental R. pneumotropicus infection. A mild to moderate interstitial pneumonia was found in all mice including controls and sentinels. Contact and bedding sentinels showed no clinical signs and pathologies related to R. pneumotropicus infection (data not shown).

Mortality (a) and body weight (b) of the indicated mice infected with R. pneumotropicus JF4Ni (n = 16 per mouse strain) or treated with PBS as control (n = 10 for BALB/c and n = 9 for C57BL/6, one control died during anaesthesia). Data of contact sentinels are not included. Bronchopneumonia was a main pathology. A multifocal severe catarrhal-purulent bronchopneumonia of a BALB/c mouse 2 days after intranasal infection is shown (c). Alveoli and bronchioles of this mouse were infiltrated with high numbers of neutrophilic granulocytes (200 x magnification). The log rank test was used to analyse differences between the two mice strains and the groups (a)

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Detection of R. pneumotropicus in tracheonasal lavages (TNL) and internal organs

R. pneumotropicus was detected in TNL and various internal organs of experimentally infected animals. Furthermore, this pathogen disseminated into non-respiratory internal organs in every experimentally infected mouse (Fig. 2). Bacterial loads in the brains, lungs, L n. tracheobronchiales, livers, spleens, kidneys and genito-urinary tracts were significantly higher in BALB/c than in C57BL/6 mice as assessed by semi-quantitative scoring (mean bacteriological scores for mice succumbing to infection: BALB/c: 11.6 with SD 3.0 and C57BL/6: 6.1 with SD 1.9; p = 0.002; Additional file 1: Table S1; Fig. 2). In contact sentinels R. pneumotropicus was mainly detected in the lungs and TNLs (Fig. 2), indicating that dissemination occurred mainly in experimentally infected animals but not in contact sentinels. Additionally, R. pneumotropicus was not detected in bedding sentinels at all.

Semi-quantitative determination of R. pneumotropicus in the indicated tissues of BALB/c (a) and C57BL/6 (b) mice either infected experimentally (losses and survivors) or used as contact sentinels. Losses occured 2–6 dpi, survivors were sampled 28 dpi and contact sentinels 56 dpi. A low grade is equal to less than 20 CFU per plate; a middle grade refers to 20–70 CFU and a high grade to more than 70 CFU per plate

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BALB/c and C57BL/6 mice succumbing to infection within 2 to 6 days post infection (dpi) had high specific bacterial loads in TNL in most cases (mean of 2.6 × 10⁶ colony forming units (CFU)/ml with SD 3.1 × 10⁶ and 3.4 × 10⁵ CFU/ml with SD 3.7 × 10⁵, respectively). At the end of the observation period, the bacterial load of the lung was significantly higher in surviving BALB/c mice than in C57BL/6 mice (mean of 4.4 × 10⁴ CFU per g tissue with SD 3.2 × 10⁴ and mean of 3.9 × 10³ CFU per g tissue with SD 5.0 × 10³, respectively, Fig. 3a). In contact sentinels, mean R. pneumotropicus loads in TNL of 2.8 × 10⁴ CFU per ml TNL in BALB/c and 2.6 × 10⁴ CFU per ml TNL in C57BL/6 were recorded (SD 3.9 × 10⁴ and 1.9 × 10⁴, respectively). Noteworthy, the mean bacteriological score based on semi-quantitative assessment of bacterial loads in the brains, lungs, lymphonodi tracheobronchiales, livers, spleens, kidneys and genito-urinary tracts was significantly higher in surviving BALB/c than in surviving C57BL/6 mice (mean bacteriological scores of 5.7 (SD 2.7) and 2.4 (SD 3.4) in BALB/c and C57BL/6 mice, respectively; p = 0.036; Additional file 2: Table S2; Fig. 2).

Quantitative determination of R. pneumotropicus in TNL and lungs of the indicated mice surviving experimental infection (a) and pathogen-specific IgA-levels in TNL (b). Medians are marked by the horizontal line. The non-parametric Mann-Whitney test was used for statistical analysis (** for P ≤ 0.01)

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Antigen-specific IgA in TNL of experimentally infected animals and sentinels

As R. pneumotropicus was isolated in TNL of experimentally infected mice surviving to the end of the observation period, we asked if this colonization occurred in the presence of specific IgA. R. pneumotropicus-specific IgA was not detected in TNL of controls and mice that died within 6 days following experimental infection. On the other hand, TNLs collected 4 weeks post infection from experimentally infected mice of both strains and BALB/c contact sentinels revealed mean titers above 80 ELISA units and mainly positive IgA-titers against R. pneumotropicus (Fig. 3b). In contrast, C57BL/6 contact sentinels had rather low specific IgA titers (mean titer of 8 ELISA units with a SD of 5.9). In summary P. pneumotropicus was found to colonize efficiently respiratory mucosa despite the presence of specific IgA in mice surviving experimental infection.

Serum IgG-levels in experimentally infected animals and sentinels

Experimental infection of BALB/c and C57BL/6 mice elicited specific IgG-titers in all surviving animals (sampled 28 dpi) as well as in contact sentinels (sampled 56 dpi) as shown by ELISA using whole cell extract or a concentrated culture supernatant as antigen (Fig. 4a and b). Sera collected prior to infection (n = 59) and from control animals (n = 19) consistently gave negative results. Furthermore, R. pneumotropicus-specific IgG was not recorded in sera from mice succumbing to infection within the first 6 dpi or in sera from bedding sentinels.

IgG-levels against the indicated R. pneumotropicus antigens in intranasally infected BALB/c (a) and C57BL/6 (b) mice and the respective contact and bedding sentinels in sera drawn at the indicated time points. A serum pool from mice naturally infected with R. pneumotropicus was used as reference serum. The culture supernatant had a concentration factor of 100. Early losses refer to mice killed for animal welfare reasons after developing severe signs of sepsis. Statistical analysis with the Mann-Whitney test was performed to analyse differences between the different groups. The Wilcoxon test was used to compare different time point values within the same groups. The star in panel (b) (whole cell extract) indicates significance (* for P ≤ 0.05)

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IgG subclass differentiation indicate differences in the immune response of BALB/c and C57BL/6 mice to R. pneumotropicus infection

As the specific bacterial load of the lung of surviving BALB/c mice was significantly higher than the load of C57BL/6 mice (Fig. 3a), we investigated putative differences in the immune response of the two mice strains. We used levels of IgG subclasses as indicators for the kind of immune response as IgG2a and IgG2b are associated with a Th1 response while IgG1 is associated with a Th2 response. Upon infection, not only the ratio of antigen-specific IgG subtypes might change in serum in association with a Th1 or Th2 response, but also the overall ratios of IgG subtypes [24]. Differentiation of IgG subclasses was conducted in 7 BALB/c and 8 C57BL/6 mice showing a distinct antibody response to R. pneumotropicus antigen. In BALB/c mice, we measured the ratios of IgG2a to IgG1 and IgG2b to IgG1. Due to the lack of IgG2a in C57BL/6 mice [25] only the ratio of IgG1 to IgG2 in was determined in this strain. Prior to infection, the mean IgG2/IgG1 ratios were 0.5 for IgG2a and 0.4 for IgG2b in BALB/c and 0.8 for IgG2b in C57BL/6 mice (Fig. 5a and b). Post infection, the mean IgG2a/IgG1 ratio in BALB/c mice increased slightly to 0.7, while the IgG2b/IgG1 ratio remained constant. These results indicate a balanced immune response with a tendency to Th2 in BALB/c mice. In C57BL/6 the IgG2b to IgG1 ratio increased to 1.6 indicating a Th1 prone immune response (Fig. 5a). Accordingly, the majority of surviving, experimentally infected C57BL/6 mice had high R. pneumotropicus-specific IgG2c titers (above 50 ELISA Units), whereas these antibodies were not recorded in sera drawn from these mice prior infection or from control mice (Fig. 5c).

Ratios of the indicated IgG-subclasses in surviving C57BL/6 (a) and BALB/c (b) mice and antigen-specific IgG2c titers in respective C57BL/6 (c). Seven infected BALB/c and 8 C57BL/6 mice with a distinct antibody answer to R. pneumotropicus antigen (Fig. 4) were chosen for the determination of IgG subclasses in (a) and (b), respectively. In BALB/c mice the ratios between IgG2a to IgG1 and IgG2b to IgG1 were determined. As C57BL/6 mice lack IgG2a, only IgG1 and IgG2b were measured. Medians are marked by the horizontal line. Differentiation of a Th1 and Th2 immune response is indicated by the dashed line. IgG2c-titers in C57BL/6 mice against whole cell extract of R. pneumotropicus (c). Titers were determined as indicated either in experimentally infected survivors or respective controls (fbl = final bleeding). A serum pool from C57BL/6 mice naturally infected with R. pneumotropicus was used as reference serum. The non-parametric Mann-Whitney test was used for statistical analysis. The P-values are indicated

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Experimental infections with P. pneumotropica have been conducted in vaccination studies to investigate the protective efficacies of different recombinant proteins such as the RTX toxin PnxIII [9] and different outer membrane proteins [26]. In these studies, protective efficacies were assessed by determining specific bacterial loads at different mucosal sites such as the nasal conchae, lung and conjunctivae. However, clinical read out parameters were not included. Here, an infection model with high rates of morbidity and mortality in immunocompetent BALB/c and C57BL/6 wildtype mice was established for the first time, enabling the usages of respective read out parameters in future vaccination studies. The high morbidity was associated with severe lung pathologies and dissemination of R. pneumotropicus to extra-respiratory sites such as liver and brain. Based on the presented data we consider these models as ideal for investigating protection against severe pneumonia and associated sepsis. Importantly, numerous immunogens of R. pneumotropicus are homologous to proteins expressed by Haemophilus influenza [26] and P. multocida [26], two important pneumonia and sepsis agents in humans and livestock, respectively. Thus, vaccination trials using the described murine models might be relevant for these pathogens as well. The fact that mice are the natural host of R. pneumotropicus is an important advantage, especially as members of the Pasteurellaceae show substantial host adaptation.

The infection dose of 1 × 10⁸ CFU used in this study is high. However, previous studies have used similar or even higher [15, 27, 28] doses without induction of morbidity and mortality. For example, Chapes et al. could not induce any clinical signs or pathologies in immunocompetent C57BL/6 wildtype mice with a 400 times higher dose of the R. pneumotropicus type strain ATCC 35149 [27]. Furthermore, immunocompetent Crlj:CD1 mice did not develop lung lesions or clinical signs of disease after experimental infection with the R. pneumotropicus type strain in contrast to immunodeficient NOD/ShiJic-scid/Jcl mice [28]. This difference to previous studies might be related to differences in virulence between R. pneumotropicus strains. The R. pneumotropicus JF4Ni strain used in this study is regarded as highly virulent based on the results of the experimental infections and the substantial health issues of the animal facility it was detected in. The fact that this strain bears all three known RTX toxin genes of this pathogen might be related to its virulent phenotype as the toxins are considered important virulence factors [8,9,10]. Specifically, PnxIII is cytotoxic to macrophages [10], which are crucial for clearance of R. pneumotropicus in the lungs as shown by transfer of Toll-like receptor 4-positive macrophages to knockout mice [29]. Noteworthy, more than 70% of the R. pneumotropicus strains investigated in this study shared this RTX toxin genotype, namely pnxIA+ pnxIIA+ pnxIIIA+. As these strains were recently isolated, putative emergence of this important pathotype should be further investigated.

All surviving animals of both mouse strains and their contact sentinels produced high levels of R. pneumotropicus-specific IgG antibodies, as shown by ELISA using two different antigens. Sera drawn prior to infection and from control animals consistently gave negative results which indicates high specificities of the established ELISAs. Noteworthy, a commercially available ELISA for the detection of P. pneumotropica-specific IgG failed to detect specific antibodies in the sera of infected animals surviving until the end of the experiment (results not shown).

In agreement to previous studies, all bedding sentinels were serologically negative, rendering this approach inappropriate for R. pneumotropicus health monitoring [21, 23]. On the other hand, serological screenings of contact sentinels for R. pneumotropicus-specific serum IgG using the described ELISA seems to be rather sensitive as an indirect indicator of infection and specific based on the results shown in Fig. 4. Furthermore, contact sentinels might be useful to study clinically inapparent colonization, as none of these mice became morbid at any time post infection despite colonisation of the lungs in numerous animals (Fig. 2).

This study shows for the first time that R. pneumotropicus infection results in a mean ratio of IgG2b to IgG1 above 1 in C57BL/6 but not in BALB/c mice indicating a Th1-prone immune response. In contrast, IgG2/IgG1 in BALB/c mice remained below 1 post infection suggesting a more balanced response. It is known already that BALB/c and C57BL/6 mice exhibit distinct genetically determined differences in their immune systems under physiological conditions, which includes higher amounts of interleukin (IL)-12 in C57BL/6 [30] and associated higher productions of IgG2c and 2b [31] inducing a Th1 immune response. However, based on the rapid progress of disease starting very early after infection, it is reasonable to hypothesize that other mechanisms but Th1 and Th2 immune responses were crucial for survival in the immunologically naïve mice of the described experimental infection. This is in agreement with the finding that the more Th1-prone C57BL/6 and the more Th2-prone BALB/c mice show comparable morbidities and pathologies.

We found high titres of R. pneumotropicus-specific IgA (above 150 Elisa) in the TNL of two surviving BALB/c mice 28 dpi in association with high numbers of this pathogen (above 10⁴ CFU/ml, results not shown). These results suggest maintenance of mucosal colonization of R. pneumotropicus despite high titers of specific IgA. As the specific bacterial load in the lung of the investigated survivors was significantly lower in C57BL/6 than in BALB/c mice, it is reasonable to hypothesize that the putative Th1-prone immune response in C57BL/6 mice is more efficient in restricting persisting lung infection.

Many R. pneumotropicus strains recently isolated from laboratory mice in Germany carry the genes of the three known RTX toxins of this pathogen. Intranasal application of the pnxIA+ pnxIIA+ pnxIIIA+ R. pneumotropicus JF4Ni strain results in invasive and fatal infections in wt BALB/c and C57BL/6 mice associated with severe pneumonia and dissemination to extra-respiratory sites. In contrast to BALB/c mice, surviving C57BL/6 mice show a Th1-prone immune response and a bacterial load of the lung below 10⁴ CFU per g tissue after 28 dpi. The described model is ideal for future studies on virulence and protection elicited by vaccination.

Animals

Eight-week-old female wild type BALB/c mice obtained from Charles River laboratory (Sulzfeld Germany) and C57BL/6 mice from Janvier Labs (Le Genest-Saint-Isle France), both specific pathogen free, were caged randomly in 6 groups per strain including 2 uninfected and 4 infected groups. Each group contained 4 infection/placebo treated animals and one contact sentinel. Additionally, 10 week old female P. pneumotropica-free CD1 outbred mice (raised by the Fraunhofer Institute for Cell Therapy and Immunology, Leipzig, Germany) were included in this study as bedding sentinels (2 cages with 4 mice each). Each bedding-group was assigned to one mouse strain. The number of animals included in this study was based on the objectives to reveal putative differences between BALB/c and C57BL/6 mice in susceptibility, to evaluate sentinel monitoring and to obtain convalescence sera for a further immunoproteomics study. All animals were housed as described in a previous study in detail [32], which included ventilated cages with HEPA filters and air conditioning as well as ad libitum feeding and drinking. One week before infection blood samples were collected from the submandibular vein and stored at − 20 °C.

Bacterial strains and culture media

R. pneumotropicus and R. heylii were cultivated as appropriate overnight at 37 °C on Columbia Blood Agar (COB) or in Brain Heart Infusion (BHI). Experimental infection was conducted with R. pneumotropicus strain JF4Ni grown in BHI until a concentration of 10⁸ colony forming units (CFU) per millilitre was reached. This strain was recently isolated from a German research facility with severe health problems associated with dyspnoea and increased mortality in P2X₂/P2X₃^Dbl−/− knockout but also wt mice [33]. Furthermore, R. pneumotropicus reference strain ATCC 35149 and 27 Biotype Jawetz- as well as 26 Biotype Heyl strains were included in this study (Additional file 3: Table S3).

Infection

For experimental infection/mock treatment mice were anaesthetised by isoflurane inhalation. Mice were experimentally infected by intranasal application of 1 × 10⁸ CFU R. pneumotropicus JF4Ni in 25 μl phosphate buffered saline (PBS, 12.5 μl per nostril). Controls were inoculated with PBS only. Contact sentinels remained untreated, bedding sentinels were turned over to used bedding 7 days after inoculation. Experimentally infected and sentinel animals were sacrificed 4 and 8 weeks after experimental infection, respectively. For this, mice were anaesthesized through intraperitoneal application of 100 mg ketamin per kg body weight and 5 mg xylazin per kg body weight. They were bled by heart puncture and finally killed by cervical dislocation.

Clinical examination and treatment

Every 12 h thorough adspection and weighing of mice was performed. Based on predefined criteria (Additional file 4: Table S4) clinical signs were scored. Mice with a cumulative clinical score of 3 or more were treated with flunixin meglumine for animal welfare reasons (5 mg per kg body weight every 12 h subcutaneously). The following end points led to euthanasia of respective animals: bleeding from orifices, paralysis, acute respiratory distress, cyanosis and 20% weight loss. Mice with a cumulative score above or equal 9 or a score above or equal 6 for 24 h were also killed for animal welfare reasons.

Pathological examinations

For pathological studies brain, nasal conchae, lung, liver, spleen and kidney were collected, macroscopically examined and fixed in 4% CaCO₃ buffered formalin. Tissues were embedded in paraffin, sectioned and stained with haematoxylin and eosin for light microscopy. Scoring of histopathological findings was conducted as specified in Additional file 5: Table S5.

Cultural examinations

For semi quantitative cultural examinations, lung, brain, lymphonodi tracheobronchiales, liver, spleen, kidney and the genito-urinary tract of all BALB/c and C57BL/6 mice were collected and a fresh cut side was pressed on a COB plate, which was incubated for 24 h at 37 °C after streaking. For comparative analysis low, middle and high grades of detection of the typical colonies were scored with 1, 2 and 3 for each investigated tissue, respectively. The sum of the scores for all investigated tissues constitutes the total bacteriological score of each animal. Furthermore, quantitative cultural examinations were performed with the TNLs (300 μl PBS). For this, TNLs were serially diluted, spread on COB in duplicates and incubated for 24 h at 37 °C. Colonies were differentiated by MALDI-TOF-MS (Bruker microflex LT, Bremen).

Antigen preparation and ELISA for detection of antigen-specific serum-IgG, serum-IgG2c and mucosal IgA

ELISAs were established for detection of serum IgG and mucosal IgA directed against R. pneumotropicus antigen. Either a whole cell extract or a concentrated culture supernatant of R. pneumotropicus JF4Ni was used as antigen.

For preparation of the antigens, 100 ml R. pneumotropicus culture were centrifuged at 2000 g for 15 min at 4 °C. The supernatant was concentrated 100 fold with a 30 kDa centrifugal filter unit (Amicon ultra), mixed with 0.5 ml 10 x protease inhibitor (Protease Inhibitor Cocktail with EDTA by Sigma Aldrich) per g cell pellet and dialyzed against 0.9% NaCl.

Whole cell extract was prepared from pelleted bacteria as described for Streptobacillus moniliformis previously [32]. Three hundred nanogramms of P. pneumotropica antigen (either whole cell extract or a concentrated culture supernatant) or casein (background measurement) were used per well to coat Corning Costar® assay plates in carbonate buffer (pH 8.1). Blocking with casein and washing of ELISA plates was conducted as described [32]. Twofold serial dilutions of sera and TNLs in PBS with 2 mM EDTA, 0.1% Tween20 and 0.1% bovine casein were applied to the ELISA plates including also reference sera/reference TNLs as well as negative controls. For detection of P. pneumotropica-specific serum-IgG, serum-IgG2c or TNL-IgA, plates were incubated for 1 h at RT with a 1:10,000 dilution of a HRP-conjugated goat anti-mouse IgG antibody (Jackson Immuno Research Laboratories), or a 1:10,000 dilution of a HRP-conjugated goat anti-mouse IgG2c antibody (Biorad; C57BL/6 mice only) or a 1:5000 dilution of HRP-conjugated goat anti-mouse IgA antibody (BIOMOL GmbH), respectively. ELISA plates were developed with 3,3′,5,5′-tetramethylbenzidine as described [32]. Absorbance was measured at 450 nm (reference at 630 nm).

The samples and the controls were measured in a duplicate series of four (seven for reference sera) twofold dilutions (starting with 1:200 for IgG and 1:50 for IgA). Sera collected from mice of a laboratory animal facility infected with the R. pneumotropicus strain JF4Ni were pooled and served as reference in the IgG and IgGc ELISA, TNL of an experimentally infected mouse from this experiment with a mean antibody titre as reference for the IgA ELISA. These reference samples were defined to include 100 ELISA units. Pooled sera and TNL samples from R. pneumotropicus-free mice were used as negative controls. Calculation of ELISA units for IgG and IgA was conducted as previously described [34].

Determination of concentrations of IgG subtypes and respective ratios in sera of experimentally infected mice

Determination of IgG subtypes and calculation of respective ratios was conducted as described previously [32].

Purification of DNA

The DNeasy Blood & Tissue Kit (Qiagen) was used according to the manufacturer’s instruction to purify DNA from R. pneumotropicus and R. heylii cultures.

PCR screening for RTX genes pnxIA, pnxIIA and pnxIIIA

To detect the RTX toxin genes pnxIA, pnxIIA and pnxIIIA the primer pairs pnxIAF/pnxIAR, pnxIIAF/pnxIIAR and pnxIIIAF/pnxIIIARs (Additional file 6: Table S6) were used. The pnxIA and pnxIIA genes were amplified in full length from the DNA purified from different isolates (Additional file 3: Table S3), including strains genotyped in previous studies through 16S–23S rRNA internal transcribed spacer analysis [6, 35]. For detection of pnxIIIA amplification of an internal 1 kbp fragment was conducted. The pnx sequences were amplified by PCR with 30 cycles and Taq-polymerase (Invitrogen Thermo Scientific Fisher) as recommended by the manufacturer using the following conditions: denaturation at 95 °C for 30 s, annealing at 58 °C (pnxIA and pnxIIIA) or 61 °C (pnxIIA) for 30 s and elongation at 72 °C for 3:30 min (pnxIA), 6:30 min (pnxIIA) or 2 min (pnxIIIA).

Statistical analysis

The Mann-Whitney test was performed to analyse differences between the different groups of mice. The Wilcoxon test was used for comparison of different time point values within the same group. The data in the Kaplan-Meyer survival and morbidity diagrams were analysed with the log rank test. Probabilities lower than 0.05 were considered significant, lower than 0.001 highly significant.

BGPST:

5% BSA, 0.1% gelatine and 0.05% Tween20 in PBS

BHI:

Brain heart infusion

CFU:

Colony forming units

COB:

Columbia Blood Agar

dpi:

days post infection

ELISA:

Enzyme-linked immunosorbent assay

FELASA:

Federation of Laboratory Animal Science Association

IgG/A:

Immune globuline G/A

IL:

Interleukin

P. multocida :

Pasteurella multocida

P. pneumotropica :

Pasteurella pneumotropica

PBS:

Phosphate buffered saline

PCR:

Polymerase chain reaction

R. pneumotropicus/heylii :

Rodentibacter pneumotropicus/heylii

RTX:

Repeats in toxin

SD:

Standard deviation

Th:

T-helper cell

TNL:

Tracheonasal lavage

Funding

This work was financially supported by the European Funds of Regional Development (EFRE). The funding body had no role in the design of the study and collection, analysis, and interpretation of data as well as in writing the manuscript.

Availability of data and materials

The datasets analysed during this current study are available from the corresponding author upon a reasonable request.

Authors and Affiliations

1. Institute for Bacteriology and Mycology, Faculty of Veterinary Medicine, University Leipzig, An den Tierkliniken 29, 04103, Leipzig, Germany

   Juliane Fornefett, Wieland Schrödl & Christoph Georg Baums

2. Fraunhofer Institute for Cell Therapy and Immunology, Leipzig, Germany

   Jaqueline Krause & Thomas Grunwald

3. Institute for Veterinary Pathology, Faculty of Veterinary Medicine, University Leipzig, Leipzig, Germany

   Kristin Klose

4. GVG Diagnostics GmbH, Leipzig, Germany

   Felix Fingas

5. Institute of Bioanalytical Chemistry, Faculty of Chemistry and Mineralogy and Centre for Biotechnology and Biomedicine, University Leipzig, Leipzig, Germany

   Felix Fingas & Rayk Hassert

6. Central Unit for Animal Research and Animal Welfare Affairs, Heinrich-Heine-University, University Hospital, Düsseldorf, Germany

   Laurentiu Benga

7. Institute of Immunology/Molecular Pathogenesis, Faculty of Veterinary Medicine and Centre for Biotechnology and Biomedicine, University Leipzig, Leipzig, Germany

   Uwe Müller

Contributions

CB and TG conceived the study. CB, TG, UM, WS, FF and RH designed the experiments. Acquisition of data was mainly conducted by JF. The clinical screenings were also performed by JK. LB provided strains, protocols and acquired data regarding strain differentiation. The histopathological screenings were performed by KK. Data analysis was conducted by JF with support from UM, FF, RH, WS and CB. JF and CB drafted the manuscript. All authors critically revised the manuscript, approved the final manuscript and agreed to be accountable for all aspects of the work.

Corresponding author

Correspondence to Christoph Georg Baums.

Ethics approval

This animal study was registered and approved under no. TVV 17/15 at the Provincial Head Office Saxony (Germany), Unit 24, Veterinary and Food Inspection (Landesdirektion Sachsen, Referat 24, Veterinärwesen und Lebensmittelüberwachung) which includes approval through the registered committee for animal experiments. This study and handling of mice in general was conducted in strict accordance with the principles outlined in the EU Directive 2010/63/EU and German Animal Protection Law.

Competing interests

GVG Diagnostics is a diagnostic services provider. Felix Fingas is part-time employee at GVG Diagnostics.

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