key: cord-0062506-uezxgj4n authors: Yoshida, Sho; Inaba, Hiroaki; Nomura, Ryota; Murakami, Masaru; Yasuda, Hidemi; Nakano, Kazuhiko; Matsumoto-Nakano, Michiyo title: Efficacy of FimA antibody and clindamycin in silkworm larvae stimulated with Porphyromonas gulae date: 2021-04-25 journal: nan DOI: 10.1080/20002297.2021.1914499 sha: e8c78c5b130f9799e144201ff09c154c6b06ec09 doc_id: 62506 cord_uid: uezxgj4n Objective: Porphyromonas gulae, a major periodontal pathogen in animals, possesses fimbriae that have been classified into three genotypes (A, B, C) based on the diversity of fimA genes encoding fimbrillin protein (FimA). P. gulae strains with type C fimbriae were previously shown to be more virulent than other types. In this study, we further examined the host toxicity mediated by P. gulae fimbriae by constructing recombinant FimA (rFimA) expression vectors for each genotype and raised antibodies to the purified proteins. Methods and Results: All larvae died within 204 h following infection with P. gulae type C at the low-dose infection, whereas type A and B did not. Among fimA types, the survival rates of the larvae injected with rFimA type C were remarkably decreased, while the survival rates of the larvae injected with rFimA type A and type B were greater than 50%. Clindamycin treatment inhibited the growth of type C strains in a dose-dependent manner, resulting in an increased rate of silkworm survival. Finally, type C rFimA-specific antiserum prolonged the survival of silkworm larvae stimulated by infection with P. gulae type C strain or injection of rFimA type C protein. Conclusion: These results suggested that type C fimbriae have high potential for enhancement of bacterial pathogenesis, and that both clindamycin and anti-type C rFimA-specific antibodies are potent inhibitors of type C fimbriae-induced toxicity. This is the first report to establish a silkworm infection model using P. gulae for toxicity assessment. Porphyromonas gulae, a Gram-negative blackpigmented anaerobe, is the predominant species of Porphyromonas found in the periodontal pocket in dogs [1] . Characterization of P. gulae has shown it to be a major factor related to periodontal disease in dogs [2] . Recent studies have reported that P. gulae was detected in the gingiva and other periodontal tissues from healthy owners of companion animals [3, 4] , and that it invaded human gingival epithelial cells [5] . P. gulae was also shown to inhibit cell migration in mammalian cells and induce production of inflammatory cytokines, including interleukin (IL)-1β, IL-6, IL-8, and tumor necrosis factor-α [3, 6, 7] . These findings suggest that P. gulae may be involved in the development of periodontitis. Many important virulence factors, including fimbriae, proteases, endotoxins, and capsules, are involved in bacterial pathogenesis and infectious disease [8, 9] . Fimbrillin protein (FimA), the major subunit of fimbriae, is displayed on the cell surface, where it can play roles in several important functions, including the capacity to facilitate adhesion, colonization, biofilm formation, signal transduction, enzymatic degradation, and motility [5, 10, 11] . For several pathogens, including Streptococcus parasanguis, P. gingivalis and Salmonella enterica, FimA has been reported to impact bacterial pathogenesis [12] [13] [14] . The fimbriae of P. gingivalis have been classified into six genotypes (types I-V and Ib) based on the nucleotides sequences [15] . Several phenomena of the host-pathogen relationship are reportedly dependent on the fimA genotype, namely periodontal health status, bacterial adhesion to and invasion of host cells, and inflammatory induction [11,-15-17] , suggesting that clonal variations in fimbriae may be related to P. gingivalis virulence [16, 17] . P. gulae is well known as the animal biotype of the human periodontal pathogen P. gingivalis [18] . P. gulae fimbriae are hair-like appendages on the bacterial surface and are considered to be a critical virulence factor, mediating host tissues adherence and invasion [3] . Fimbriae from both P. gulae and P. gingivalis are classified into three major genotypes: A, B and C, with type C showing high virulence for periodontal disease, followed by B and then A [3, 4, 7] . P. gulae with type C fimbriae also exhibit greater levels of virulence in animal and human host cells compared with the other genotypes [4, 7, 19, 20] . These reports suggest that the virulence of P. gulae may depend, to some extent, on the clonal diversity of fimbriae. However, the interaction between P. gulae infection and toxicity in an in vivo model has yet to be investigated. The present study is the first to describe the silkworm P. gulae infection model, in which we examined optimal conditions for the assessment of virulence, and analyzed antibiotics sensitivity and response to anti-rFimA-specific antibodies. Bacterial culture conditions P. gulae strains ATCC 51700 (fimA type A) [7] , D040 (fimA type B) [7] , and D049 (fimA type C) [3] were used in this study. Each strain was isolated from an oral swab specimen from a dog and confirmed to be P. gulae using a molecular biological method described previously [3] . P. gulae strains were cultured in Trypticase soy broth (Becton, Dickinson and Co., Franklin Lakes, NJ, USA) supplemented with yeast extract (1 mg/ml), hemin (5 µg/ml), and menadione (1 µg/ml), as described previously [5] . Escherichia coli DH5α (Nippon Gene, Tokyo, Japan) and E. coli BL21 (Nippon Gene) were used as host strains for transformation of plasmid DNA. E. coli strains were grown in Luria-Bertani (LB; 1% tryptone, 0.5% yeast extract, 0.5% NaCl) medium; LB agar was prepared by the addition of 1.5% agar. When necessary, kanamycin sodium (100 µg/ml) was added to the medium. P. gulae genomic DNA was isolated as previously described [3] and used as a template for amplifying the entire fimA gene by PCR. The primers used for PCR were constructed from the sequences of the fimA genotypes [3] as follows: type A forward primers, 5′-GCG CGC GAA TTC GAG ATG AAA AAG ACT AAG-3′ and reverse primers, 5′-GCG CGG TTT AAG CTT TGA TTA CCA AGT AGC-3′; type B forward primers, 5′-GCG AAC GGA TCC AAG ATG AAA AAG ACT AAG-3′ and reverse primers, 5′-CGC TCT CTC GAG AGC TGA TTA CCA AAT-3; type C forward primers, 5′-ATC GAT ATC CAC TTT TAA AAC AAA AAA GAG-3′ and reverse primers 5′-TTT AGT CGT TTG ACG GGT CGA TTA CCA AGT-3′. Each amplified DNA was cloned into pGEM-T Easy Vector (Promega, Madison, WI), then digested with the appropriate restriction enzyme for ligation into the pET 42a (+) glutathione S-transferase (GST) gene fusion-protein expression vector (Novagen, Madison, WI, USA). The ligated vector was transformed into E. coli DH5α and colonies were selected on LB agar plates containing 50 µg of ampicillin/ ml. Plasmid DNA was obtained using the Wizard® Plus SV Minipreps DNA Purification System (Promega). Each recombinant plasmid was transformed into E. coli BL21 (DE3) (Nippon Gene) and the colonies were selected as described above. Production of each rFimA was induced with isopropylb-D-thiogalactopyranoside (IPTG), and the proteins were purified using a modification of a method described previously [21] . Briefly, an overnight culture (10 ml) of each transformed BL21 strain was used to inoculate 500 ml fresh LB broth containing 50 μg ampicillin/ml. The cultures were incubated at 37°C with vigorous shaking until the optical density at 600 nm reached 0.6, and then IPTG was added to a final concentration of 1 mM. After an additional 3 h of incubation to induce GST-rFimA fusion proteins, the cells were harvested by centrifugation at 2000 × g for 15 min at 4°C, and washed three times with phosphate-buffered saline (PBS) buffer. The cell pellets were suspended in the same buffer and ultrasonicated on ice. Supernatants were obtained by centrifugation and purified using a glutathione Sepharose™4B column (GE Healthcare, Fairfield, CT, USA). The purified GST-rFimA fusion proteins were subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and stained with Coomassie blue (Figure 1a ). The purified proteins were dialyzed with MilliQ and freeze-dried. Rabbit anti-rFimA antibodies were generated using a method described previously [21] . Purified rFimA protein was mixed with a block copolymer adjuvant (Titer-Max Gold; CytRx Co., Atlanta, GA, USA) and injected intramuscularly into adult New Zealand white rabbits weighing 1-1.5 kg (Oriental Yeast Co. Ltd., Tokyo, Japan) twice with a 14-day interval. One week after the second injection, blood was drawn, and antisera were collected and stored at −20°C. The antisera were separated by SDS-PAGE, transferred to a polyvinylidene fluoride membrane, and probed with anti-GST antibody to confirm the GST-rFimA antibody titers (Figure 1b) . We used the following antibiotics: from Sigma (St. Louis, MO, USA), gentamicin and metronidazole; from Wako (Osaka, Japan), ampicillin and clindamycin. Freshly cultured P. gulae in the exponential phase of growth were employed so that antibiotics reactions could be observed for 24 h. Bacterial growth was measured on an SH-1000 Lab microplate reader (Corona Electric, Ibaraki, Japan) at 595 nm. The silkworm infection experiments were performed as described previously [22] . Briefly, silkworms were raised from fertilized eggs to four-instar larvae in our laboratory. The hatched four-instar larvae were fed antibioticfree food (SilkMate 2S, Nosan Corporation, Kanagawa, Japan) for 1 day. P. gulae suspensions (1 × 10 7 or 5 × 10 7 colony-forming units [CFU] in 50 μl PBS) and rFimA protein (5 µg in 50 μl) were injected into the silkworm hemolymph through the dorsal surface of the silkworms (n = 10) using a 26-gauge needle (Terumo, Tokyo, Japan). After injection, larvae were incubated at 37°C and their survival rate was measured every 24 h for 240 h. Several different concentrations of rFimA protein were preliminarily examined to determine the concentration used in this study (Supplementary Figure 1 ) with 5 µg determined as the appropriate concentration for comparing protein efficacy. A P. gulae suspension (5 × 10 7 CFU in 50 μl PBS) or rFimA protein (5 µg in 50 μl) was injected into the hemolymph of the silkworms (n = 10) using a 26gauge needle (Terumo), and immediately followed by the injection of clindamycin and anti-rFimA specific antisera. The survival rate was assessed every 24 h for 240 h after injection. Statistical analyses were performed using the computational software packages StatView software (version 5.0, SAS Institute Inc., Cary, NC, USA). Student t-test was utilized to compare the effect of each antibiotic. Survival rates of the silkworm larvae in each group were evaluated with a Kaplan-Meier plot, which was analyzed by a log-rank test. A P value of <0.05 was considered to be statistically significant. We generated recombinant versions of all three fimA genotypes of P. gulae to determine the virulence of each. The molecular sizes of the rFimA proteins were all approximately 75 kDa (Figure 1a ). We also generated antisera against the rFimA proteins and used western blotting to show that each antiserum reacted with its corresponding purified rFimA (Figure 1b ). In addition, an enzyme linked immunosorbent assay (ELISA) was performed to analyze the results of each anti-rFimA assay (Supplementary Figure 2) . Those findings demonstrated no cross-reactions and that specific results were obtained. Silkworm larvae have been characterized as an animal model of human infection with pathogenic bacteria [23] . Thus, we established and examined a P. gulae infection model using silkworm larvae. Figure 2 shows that, although 30% of the control larvae had died at 204 h under treatment with PBS, all of the larvae died within 204 h following infection with P. gulae D049 (type C) at the low dose (1 × 10 7 CFU); by contrast, infections with P. gulae ATCC51700 (type A) and P. gulae D040 (type B) at the same dose were less virulent (Figure 2a) . High-dose infection (5 × 10 7 CFU) of P. gulae was found to eliminate the entire silkworm population at 144 h (Figure 2b ). By comparison, at 228 h after a high-dose infection with types A and B, 10% of the larvae infected with P. gulae type A were still alive, while all of the larvae infected with P. gulae type B had died (Figure 2b ). When larvae were injected with purified rFimA proteins, by the end of the experiment (240 h), the survival rates of those injected .Inhibitory effects of antibiotics on the growth of P. gulae. P. gulae (5 × 10 7 CFU) was cultured in trypticase soy broth TSB and an antibiotic at the concentrations indicated for 24 h. after incubation, bacterial growth was measured using a microplate reader. Data are expressed as the relative ratio of treated/untreated cultures and represent means ± SD from three independent experiments analyzed with a t-test. *P < 0.05; **P < 0.01; ***P < 0.001. with all the rFimA proteins were lower as compared to those injected with GST only as well as the PBS control. Also, most (~90%) of the larvae injected with rFimA type C died, whereas the survival rate of larvae injected with rFimA type A or B exceeded 50% (Figure 3 ). We considered that this effect was caused by immune response and not cell disruption by a massive dose of recombinant proteins, since the survival rate of larvae injected with GST was only higher as compared to that received all recombinant proteins. These findings suggested that strains possessing type C fimbriae are more virulent in silkworm larvae than strains possessing type A or type B fimbriae. A recent investigation demonstrated the minimum inhibitory concentrations of antibiotics against Porphyromonas spp. and Fusobacterium spp. isolated from dogs [24] , which was used to estimate the antimicrobial susceptibility of the examined P. gulae strains (Figure 4) . Clindamycin appeared to be the most effective against P. gulae, even at low doses ( Figure 4a ); by contrast, high dose of ampicillin, metronidazole and gentamicin were required to show similar levels of bacterial growth inhibition (Figure 4b-d) . Previously reported findings indicated that metronidazole and gentamicin may offer a potentially useful therapeutic option for the treatment of Porphyromonas and Prevotella spp. infections [25] . Together with the present findings, it is suggested that clindamycin may be more effective against P. gulae strains as compared to ampicillin. Inhibition of P. gulae by clindamycin led us to predict that clindamycin would improve survival of silkworm larvae infected with P. gulae. Initially, the inhibitory effects of a range of clindamycin concentrations on survival rates of larvae infected with P. gulae with type C fimbriae were examined and those results made it clear that clindamycin was effective against that infection ( Figure 5 ). The survival rates of infected larvae improved in a concentration-dependent manner (Supplementary Figure 3) . When we compared the effects of clindamycin on survival rates of infection with strains with all three fimbriae types, we found that the effect on type A infection was negligible, whereas survival of larvae infected with type B and type C strains was significantly improved (Figure 6 ). These results suggested that, of the four antibiotics tested, clindamycin may be the most effective against P. gulae-mediated infectious disease. The virulence of bacterial fimbriae has been shown to be diminished by the use of anti-FimA antibodies [11, 26] . Thus, we investigated the effect of antibodies generated against P. gulae rFimA proteins in the silkworm infection model. First, we examined a range of concentrations of type C rFimA antisera (1 to 1:1000 dilution) for their effects on the survival of injection of rFimA proteins. The most effective level of protection occurred at a 1:10 dilution (Figure 7) , which was utilized in all subsequent experiments. Next, we examined antisera against rFimA type B and rFimA type C, and found that both improved the survival rates of larvae stimulated by the corresponding rFimA protein (Figure 8 ). When we tested each antiserum for protection of silkworms against infection with each P. gulae strain type, we found that type C and type B antibodies each conferred a survival D040 (type B) , or (c) strain D049 (type C), and a 50-μl solution of 0.4 μg/ml clindamycin, and incubated at 37°C. The survival rate was recorded for the time points indicated. PBS was used as a negative control. Data are representative of three independent experiments. Survival rates in the silkworm larvae in each group were evaluated with a Kaplan-Meier plot, which was analyzed by a log-rank test. *P < 0.05; **P < 0.01. advantage, while the effects of type A antisera were negligible ( Figure 9 ). Experiments in mammalian animal models, such as cats, ferrets, dogs, monkeys, mice and rats, have been used to assess pathogenicity, host susceptibility and virulence of microbial pathogens [27] [28] [29] [30] [31] . Microorganisms are also useful as biological agents to induce the inflammatory response and reveal mechanisms of pathogenesis in the rodent mice and rats [30, 32] . However, the use of non-human primate research raises many issues related to cost, ethics, equipment, space, facilities, animal welfare and the potential for zoonosis [30, 33] . Accordingly, recent studies have shown that non-vertebrate animal models, including Caenorhabditis elegans, Drosophila, silkworms and zebrafish, offer many advantages that make them versatile for research on bacterial pathogenesis and toxicity, and the assessment of antibiotics for infectious disease [23, [34] [35] [36] . Silkworm larvae have also been useful for the characterization of bacterial pathogenicity, and the pharmacokinetics, pharmacodynamics and toxicology of drugs [37] . Silkworm larvae are quite commercially available, easily manipulated by human hands, and large enough to be injected by the same types of syringes used for human medical purposes [37] . Furthermore, the silkworm has an innate immune system akin to that in mammals, but lacks an acquired immune system [38] . Acquired resistance to pathogenic infection in silkworms, which is similar to a booster reaction, contributes to the enhancement of the immune response [39] . Silkworm muscle contraction was previously found to be strongly associated with the innate immune system of silkworms following stimulant administration [40] . Interestingly, E. coli LPS was found to not cause silkworm muscle contraction even at high doses [41] , whereas highly purified LPS activated immune gene expression [42] , suggesting that the recombinant protein expressed by E. coli could be useful for experiments with this model. Collectively, these reports indicate a high potential for a silkworm model as a replacement for animal experiments. In the present study, silkworm larvae were established as a model for P. gulae infection, and used to assess the virulence of different strains (Figures 2 and Figure 3 ). The survival rate of silkworm larvae infected with P. gulae type C strain was lower compared with type A and type B strains (Figure 2) , and injection of larvae with rFimA type C protein also dramatically lowered the survival rate ( Figure 3 ). Our findings are consistent with several previous reports, showing virulence of P. gulae with type C fimbriae in mice and cultured host-cell models (5, 19, 20) . The pathogenicity of P. gingivalis with respect to adherence to and invasion of epithelial cells depends on FimA type specificity (13) . Our results suggested that the virulence of type C fimbriae is higher than that of other FimA types, and close relationships between each specific fimA genotypes and its pathogenesis were shown. Results presented previously indicated that limitations of lethality-based studies of virulence are related to either the microbe or host variables [43] . Several pathogens, such as Bacillus anthracis, Vibrio parahaemolyticus, and E. coli, have been reported to show lethality in animal models [44] [45] [46] . In addition, there is a possibility that a P. gingivalis virulence factor, including fimbriae, could result in decreased survival of mice [17] . Moreover, P. gingivalis has been Figure 7 .Effects of rFimA type C antisera on survival of silkworm larvae injected with rFimA proteins. Silkworm larvae (n = 10) were injected with 50 μl of each rFimA protein (5 μg each of type A, B and C) and anti-rFimA type C antisera, and incubated at 37°C. The survival rate was recorded for the time points indicated. Data are representative of three independent experiments. Survival rates in the silkworm larvae in each group were evaluated with a Kaplan-Meier plot, which was analyzed by a log-rank test. *P < 0.05; **P < 0.01. Survival rates in the silkworm larvae in each group were evaluated with a Kaplan-Meier plot, which was analyzed by a log-rank test. *P < 0.05; **P < 0.01. Figure 9 .Effect of antisera raised against each rFimA protein type on silkworm larvae infected with P. gulae strains. Larvae (n = 10) were injected with a 50 μl suspension of P. gulae (5 × 10 7 CFU) type A strain ATCC51700 (a), type B strain D040 (b), or type C strain (c), and were incubated at 37°C. The survival rate was recorded at the time points indicated. PBS was used as a negative control. Data are representative of three independent experiments. Survival rates in the silkworm larvae in each group were evaluated with a Kaplan-Meier plot, which was analyzed by a log-rank test. *P < 0.001. shown to have the ability to invade human host cells, degrade cellular focal adhesion components, and induce apoptosis in a fimA-types-dependent manner [16, 47, 48] . Recent studies have noted that P. gulae organisms express several different virulence factors, including fimbriae, LPS, and trypsin-like proteases [3, 7, 49, 50] . P. gulae LPS was found to induce inflammatory responses in human gingival epithelial cells, while cell viability was not affected [49] . On the other hand, P. gulae proteases have been reported to degrade host tissue components related to growth and proliferation, resulting in promotion of morphological changes [50] . Also, P. gulae organisms with type C fimbriae have been shown to have greater levels of virulence towards mouse and human oral epithelial cells [3, 5] . However, in vitro lethal and/or toxicity models of P. gulae fimbriae related to bacterial infection have yet to be investigated. In the present study, P. gulae type C strain with recombinant FimA type C caused a dramatic decrease in survival rate (Figures 2, Figure 3 ; Supplemental Figure 1 ). The present findings obtained with an in vivo model stimulated with fimbriae are considered to reflect those obtained with in vitro models of P. gulae as well as P. gingivalis. Together, these results suggest that type C fimbriae are a significant virulence factor of P. gulae. The silkworm infection model is also useful for evaluating antibiotics and novel therapeutically effective agents for pathogenic bacterial infection [23, 37] . The silkworm model is already being used to evaluate Staphylococcus aureus cell-wall proteins and regulatory proteins as virulence factors, as well as antibiotics for human infections with bacterial pathogens, including S. aureus, Pseudomonas aeruginosa and Vibrio cholerae [23, 51] . Clindamycin is a semisynthetic derivative of the lincosamide class of compounds used clinically to treat gram-positive bacterial infections [52] . In this study, clindamycin demonstrated effective antimicrobial action against P. gulae growth, while metronidazole showed negligible effects (Figure 4 ). In addition, the effect of clindamycin was lower concentration as compared with its ampicillin (Figure 4) . Further, administration of clindamycin during infection of silkworm larvae reduced the growth of P. gulae ( Figure 6 ). Furthermore, the survival time of silkworm larvae injected with P. gulae type C was prolonged by the administration of clindamycin ( Figure 6 ). Interestingly, clindamycin was more effective against P. gulae with type C fimbriae than strains with type A or B fimbriae, indicating that functional inhibition of type C fimbriae may be an important therapeutic target for prevention of P. gulae-mediated infectious disease. A previous report noted that anti-FimA antibodies improved arthritis mediated by microorganisms [26] . In addition, adhesion of type II FimA in P. gingivalis fimbriae to epithelial cells and bacterial invasion of cells were almost completely inhibited by anti-type II FimA antibodies [11] , demonstrating the efficiency of anti-FimA antibodies for the reduction of P. gingivalis pathogenesis [11] . In the present study, the administration of rFimA antibodies prolonged the survival times of larvae infected with P. gulae (Figures 7-9 ). Together, these results suggested that our silkworm P. gulae infection model is suitable for the assessment of therapeutic effectiveness of antimicrobial reagents, such as antibiotics and antibodies. In conclusion, we established a silkworm P. gulae infection model that could be useful for the assessment of candidate therapeutic agents. Furthermore, the prolongation of silkworm survival by administration of anti-rFimA antibodies could lead to the development of new therapies for periodontal diseases. Clindamycin is a candidate with therapeutic potential for anti-host-toxicity mediated by P. gulae colonization in periodontal disease. 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We also thank Michelle Kahmeyer-Gabbe, PhD, from Edanz Group (https://en-author-services.edanzgroup.com/ ) for editing a draft of this manuscript. No potential conflict of interest was reported by the author(s). This study was supported by a Grant-in Aid for Scientific Research (B) 20H03897 and for Young Scientists (B) 19K19266 from the Japan Society for the Promotion of Science.