Pasteurella multocida capsular: lipopolysaccharide types D:L6 and A:L3 remain to be the main epidemic genotypes of pigs in China

Pasteurella multocida is a leading cause of respiratory disorders in pigs. This study was designed to understand the genotypical and antimicrobial resistant characteristics of P. multocida from pigs in China. To achieve this, we briefly investigated 158 P. multocida isolates from pigs with respiratory disorders in China between 2019 and 2020. Genotyping through multiplex PCR assays assigned these 158 isolates into capsular genotypes A (60.13%, 95/158), D (35.44%, 56/158), F (4.43%, 7/158), and/or lipopolysaccharide (LPS) genotypes L3 (28.48%, 45/158) and L6 (66.46%, 105/158). In addition, eight isolates (5.06%, 8/158) were found to be nontypable using the LPS genotyping method. When combining the capsular genotypes and the LPS genotypes, D: L6 (34.81%, 55/158) and A: L6 (31.65%, 50/158) were the predominant genotypes, followed by A: L3 (24.05%, 38/158). PCR detection of virulence factor-encoding genes showed that over 80% of the isolates were positive for exbB, tonB, exbD, ompH, ptfA, fimA, sodA, sodC, fur, ompA, oma87, plpB, hsf-2, nanH and hgbB, suggesting the presence of these genes were broad characteristics of P. multocida. We also found approximately 63.92% (101/158), 51.27% (81/158), 8.86% (14/158), 7.59% (12/158), 3.16% (5/158), 0.63% (1/158), and 0.63% (1/158) of the isolates grew well in media with the presence of colistin (4 μg/mL), tetracycline (16 μg/mL), tigecycline (1 μg/mL), ampicillin (32 μg/mL), chloramphenicol (32 μg/mL), cefepime (16 μg/mL), and ciprofloxacin (1 μg/mL), respectively. This study contributes to the understanding of genotypes and antimicrobial resistance profile of P. multocida currently circulation in pigs of China. Supplementary Information The online version contains supplementary material available at 10.1186/s44149-021-00031-7.

Pasteurella multocida is a multiple host gram-negative pathogen and a leading cause of pig respiratory disorders in the world (Peng et al. 2019a). Previously, two serotyping systems were developed based on the bacterial capsular antigens or the lipopolysaccharide (LPS) antigens which assigned P. multocida isolates into five serogroups (A, B, D, E and F) (Carter 1955) and/or 16 serovars (serovars 1~16), respectively (Heddleston et al. 1972). The application of these two serotyping systems in epidemiological studies has helped to address the serotypes of P. multocida circulating in different host species and their correlations to the diseases caused by the agent, thereby contributing to the vaccine development (Singh et al. 2014;Shivachandra et al. 2011;Dabo et al. 2007;Takashima et al. 2001). However, these two serological methods require high-quality antisera which are very difficult to be prepared and therefore it is not convenient their application in veterinary clinic (Peng et al. 2019a). Recently, the development of two multiplex PCR assays assigned the five capsular serogroups into five genotypes (A, B, D, E and F) (Townsend et al. 2001) and/or the 16 LPS serovars into eight LPS genotypes (L1~L8) (Harper et al. 2015). Based on the outcomes of these two multiplex PCR assays, we previously have established a typing system to assign P. multocida isolates from different host species into capsular: LPS genotypes (Peng et al. 2019a;Peng et al. 2018a;Peng et al. 2018b;Lin et al. 2021), and we have determined that a capsular: LPS genotype D:L6 is the most prevalent types in pigs in China according to our molecular investigation on 115 P. multocida isolates from the lungs of pigs with respiratory disease in China in 2015 (Peng et al. 2018b). Now 5 years have passed by, considering the distribution and prevalence of P. multocida serotypes (or genotypes) may vary considerably over time in a given region (Tang et al. 2009), continuously investigating and monitoring P. multocida genotypes in pigs of China is meaningful for understanding the latest epidemiological profiles of P. multocida in Chinese pig farms, which is also beneficial for the development of effective vaccines against P. multocida infections. Therefore, we undertook a separate project to determine the current profiles of capsular: LPS genotypes of P. multocida isolates in pigs of China in recent years.
To understand the capsular genotypes and LPS genotypes of swine P. multocida prevalent in pig farms of China, we investigated 158 P. multocida isolates recovered from 1371 nasal swabs and/or lungs of pigs with respiratory disorders in pig farms from 16 provinces of China between September 1, 2019 and December 12, 2020 in this study. The results reveled that types A and D were main capsular genotypes for the 158 isolates, accounting for 60.13% (95/158) and 35.44% (56/158) of the total isolates, respectively (Fig. 1A). Only two LPS genotypes were determined: L3 and L6, accounting for 28.48% (45/158) and 66.46% (105/158), respectively (Fig. 1A). In addition, eight isolates (5.06%, 8/158) were found to be nontypable using the LPS genotyping method. When combining the capsular genotypes and the LPS genotypes, D: L6 (34.81%, 55/158) and A: L6 (31.65%, 50/158) were the predominant genotypes, followed by A: L3 (24.05%, 38/158) (Fig. 1A). These genotyping results are in agreement with those of our continuously monitoring of P. multocida isolates from Fig. 1 Genotypical characteristics of P. multocida isolates from pigs of China between 2019 and 2020. A Capsular and LPS genotypes of P. multocida isolates from pigs; B Detection rates of virulence factor-encoding genes of P. multocida isolates from pigs; C Distribution of different virulence factor-encoding genes between different capsular genotypes, LPS genotypes, or capsular: LPS genotypes pigs of China from 2013 to 2017 (Peng et al. 2018b;Peng et al. 2019b) as well as our genotypical characterizations of P. multocida from different host species through the whole genome sequences (Peng et al. 2019a;Peng et al. 2018a). In particular, P. multocida capsular: LPS genotypes D: L6 and A: L3 are also prevalent in pig herds in several other regions in the world (Yeh et al. 2017;Ujvári et al. 2019). These findings suggest P. multocida capsular: LPS genotypes D: L6 and A: L3 remain to be the main epidemic genotypes in pigs of China. The capsular and LPS genotyping results of swine P. multocida recovered between 2019 and 2020, together with our previous monitoring results of swine P. multocida recovered between 2013 and 2017 (Peng et al. 2018b;Peng et al. 2019b), these nearly 10-years monitoring results indicate P. multocida capsular: LPS genotypes D: L6 and A: L3 are prevalent in pigs of China. Based on these findings, we intend to develop a multivalent inactivated vaccine against P. multocida infections in pigs.
It has been reported that P. multocida possesses multiple virulence factors contributed to the fitness and pathogenesis (Harper et al. 2006), and a large proportion of genes participated in the synthesis of these virulence factors (Peng et al. 2019a;May et al. 2001;Peng et al. 2016). Therefore, virulence genotyping based on the detection of different virulence gene profiles has also been used as a useful genotyping method (Peng et al. 2019a;Devi et al. 2018;Massacci et al. 2018;Khamesipour et al. 2014). In this study, we detected 23 kinds of virulence factors encoding genes (VFGs) that are commonly targeted in P. multocida epidemiological studies (Peng et al. 2019a;Peng et al. 2018b;Khamesipour et al. 2014 (Fig. 1B). These VFGs encoding proteins participate in bacterial colonization and adherence (ptfA, fimA and hsf-2), iron uptake and acquisition (exbB, tonB, exbD, fur and ompA), stress-resistance and self-defense (ompH, sodA, sodC, oma87, plpB, nanH and hgbB), which are widely involved in the fitness and pathogenesis of P. multocida (Peng et al. 2019a;Harper et al. 2006). Therefore, the presence of these VFGs is proposed as a common characteristics of P. multocida, with no difference between strains from different hosts or different serotypes/genotypes (Peng et al. 2019a;Peng et al. 2018a;Smith et al. 2021;Furian et al. 2016). Less than 40% of the isolates were positive for nanB (35.44%; 56/158), hgbA (27.85%; 44/158), and in particular, no isolates were positive for toxA (0.00%; 0/158), and tbpA (0.00%; 0/158) (Fig. 1B). These results are also in agreement with those from the other studies (Peng et al. 2019b;Khamesipour et al. 2014;Smith et al. 2021). toxA encodes a 146-kDa single-chain G-protein-deamidating toxin (PMT), which is commonly associated with the progressive atrophic rhinitis (PAR) (Harper et al. 2006). toxA-positive isolates are not easily recovered from pigs without obvious clinical signs of PAR (Wilson and Ho 2013). tbpA encodes the transferrin-binding protein A (TbpA), which is an important iron-uptake receptor in many gram-negative bacteria (Pogoutse and Moraes 2017). Previous articles have documented that TbpA is only possessed by P. multocida isolates from bovine species and small ruminants (Harper et al. 2006;Ewers et al. 2006). There is no difference in the distribution of different types of VFGs between different capsular: LPS genotypes, with the exception of hgbA, nanB, hsf-1, pfhA and pmHAS (Fig. 1C).
To be concluded, we found P. multocida capsular: LPS genotypes D:L6 and A:L3 are still prevalent in pigs of China . In addition, we found a large proportion of P. multocida isolates could still grow in the presence of 4 μg/mL colistin, and a proportion of isolates could grow in the presence of 1 μg/mL tigecycline. These isolates should receive more attention because Enterobacteriaceae strains with similar phenotypes are defined as colistin-and tigecycline-resistant strains, and as a potential zoonotic pathogen, treatment of multidrug resistant P. multocida might face some challenge in human medical activities.

Sample collection and bacterial isolation
Between September 1, 2019 and December 30, 2020, a total of 1371 lung samples and nasal swabs of pigs with respiratory disorders were sent by pig farms from 16 Chinese provinces to the Veterinary Diagnostic Laboratory of Huazhong Agricultural University at Wuhan, China for P. multocida detection. P. multocida isolation, purification and identification was performed as described previously (Peng et al. 2018b). Each of the P. multocida isolates recovered was finally confirmed by PCR amplifying the species-specific KMT1 gene (457 bp; Table S1 in supplementary materials) following the previously documented protocols (Townsend et al. 2001). Our previously typed swine P. multocida isolates HB03 (genotype A: L3, GenBank accession no. CP003328) (Peng et al. 2019a), HNA04 (genotype A: L6, GenBank accession no. PPVJ00000000) (Peng et al. 2018a), HN04 (genotype B: L2, GenBank accession no. PPVE00000000) (Peng et al. 2018a), HN06 (genotype D: L6, GenBank accession no. CP003313) (Liu et al. 2012), and HN07 (genotype F: L3, GenBank accession no. CP007040) (Peng et al. 2017) were used as quality-control strains in this study. Their genomic DNAs were extracted and were used as positive control for the PCR assays performed in this study.
Capsular genotyping, LPS genotyping, and virulence genotyping Capsular genotyping was performed using the multiplex PCR method described by Townsend et al. (Townsend et al. 2001). LPS genotyping was performed using the multiplex PCR method described by Harper et al. (Harper et al. 2015). Virulence genotyping was performed by PCR detection of 23 kinds of VFGs as described by Khamesipour et al. (Khamesipour et al. 2014). Primers for the genotyping of P. multocida are given in Table S1 in supplementary materials.