Detecção de genes associados à virulência em cepas de Campylobacter jejuni de origem aviária e humana

Lima, Leonardo Moreira

January 2016

A demanda por carne de frango vem crescendo globalmente, assim como as exigências com relação à qualidade microbiológica do produto final. Associa-se a frequência de Campylobacter spp. em aves às enterites em humanos. O principal reservatório do agente é o trato digestivo de animais de diversas espécies, como aves de corte. Campylobacter spp. possui ampla diversidade genotípica e fenotípica, e apresentam diversos mecanismos de virulência para se aderir e colonizar o epitélio intestinal no hospedeiro. Apesar de o controle sanitário e biossegurança implementados nas granjas refletirem na redução de contaminação das carcaças no matadouro-frigorífico, esses procedimentos não eliminam o Campylobacter completamente das aves, podendo comprometer a qualidade microbiológica do produto final e propiciar casos de toxinfecção de origem alimentar aos consumidores. Esse trabalho tem como objetivo verificar a ocorrência de seis genes de virulência de Campylobacter jejuni em amostras de carcaças de frango e em casos de campilobacteriose em humanos. Foram avaliadas 50 amostras de C. jejuni, das quais 25 eram de origem aviária, provenientes da coleção do Centro de Diagnóstico e Pesquisa em Patologia Aviária (CDPA - UFRGS), e 25 eram de origem humana, cedidas pela Fundação Oswaldo Cruz (FIOCRUZ). A técnica de reação em cadeia da polimerase (PCR) foi utilizada para detecção dos genes iam, flaA, cdtA, cdtB, cdtC e wlaN. Das amostras analisadas, 92% (23/25) de origem humana e 88% (22/25) de origem aviária foram positivas para o gene cdtB, 44% (11/25) de origem humana e 84% (21/25) de origem aviária para o gene cdtA; 20% (5/25) de origem humana e 80% (20/25) de origem aviária para o gene flaA; 48% (12/25) de origem humana e 76% (19/25) de origem aviária para o gene cdtC; 16% (4/25) de origem aviária para o gene wlaN e 12% (3/25) de origem humana e 4% (1/25) de origem aviária foram positivas para o gene iam. Em nenhuma das amostras pesquisadas de origem humana (0/25) foi observado o gene wlaN. Com este trabalho concluiu-se que os genes pesquisados podem estar presentes em cepas de C. jejuni provenientes de carne de frango e nas cepas isoladas de casos de infecção alimentar em humanos. Ainda assim, conforme os resultados apresentados, o gene cdtB teve maior frequência nas amostras provenientes de origem humana e aviária. / The demand for poultry meat has increased globally, as well as the microbiologic requirements of the final product. The frequency of Campylobacter spp. in poultry meat has been related to enteritis in humans. The digestive tract of several animals’ species, as poultries, is the main reservatory of the agent. Campylobacter spp. has a wide genotypic and phenotypic diversity, and, in addition to that, it presents several virulence factors which allow to adhere and colonize the intestinal epithelium of the host. Although good hygienic and biosecurity practices employed at poultry farms help to reduce the carcass contamination, these procedures do not completely eliminate Campylobacter spp. at the slaughterhouses and it may affect the microbiologic quality of the final product, which may cause alimentary toxinfection cases. This study aims to verify the occurrence of six virulence genes of Campylobacter jejuni from poultry carcasses samples and campylobacteriosis cases in humans. 50 samples of C. jejuni were evaluated, of which 25 were originated from poultry collected at the Centro de Diagnóstico e Pesquisa em Patologia Aviária (CDPA - UFRGS), and 25 were originated from human samples of the Fundação Oswaldo Cruz (FIOCRUZ). Polymerase chain reaction (PCR) technique was employed to detect the following genes: iam, flaA, cdtA, cdtB, cdtC and wlaN. In the samples analyzed, 92% (23/25) from human origin and 88% (22/25) from poultry for cdtB gene; 44% (11/25) from human origin and 84% (21/25) from poultry for cdtA gene; 20% (5/25) from human origin and 80% (20/25) from poultry for flaA gene; 48% (12/25) from human origin and 76% (19/25) from poultry for cdtC gene; 16% (4/25) from poultry for wlaN and gene 12% (3/25) from human origin and 4% (1/25) from poultry were positive for iam gene. This study concludes that the researched genes may be present in Campylobacter from poultry meat origin and from isolates of human cases of alimentary toxinfection. However, according to the results found, the cdtB gene had a higher frequency in samples of human and avian origin.

Qualidade microbiológica

Frango

Campylobacter jejuni

Genes

Campilobacteriose

Virulência

Virologia veterinaria : Aves

Public Health

Virulence genes

Campylobacter jejuni

Poultry Health

Campylobacteriosis

Stamm- und wirtszellabhängige Apoptose-Induktion durch Campylobacter jejuni / Strain- and host cell dependent apoptosis induction by campylobacter jejuni

Schöttelndreier, Friedrich

22 November 2011

No description available.

610 Medizin, Gesundheit

Medicine

Campylobacter jejuni

Apoptose

Cytolethal distending toxin

Cdt

campylobacter jejuni

apoptosis

cytolethal distending toxin

cdt

44.43 Medizinische Mikrobiologie

MED 331 Medizinische Mikrobiologie

Perspectives de l'usage de poudre de jaunes d’oeuf comme additif alimentaire contre Campylobacter jejuni chez le poulet : mode d'immunisation et effet de l’encapsulation

Soumaila Garba, Amina

08 1900

No description available.

Campylobacter jejuni

Colonisation

Poulet à griller

Poudre de jaunes d'œuf

Immunoglobuline

Campylobacter jejuni

Chicken colonization

Egg yolk powder

Immunoglobulin

Determination of the Structural Allosteric Inhibitory Mechanism of Dihydrodipicolinate Synthase

2015 November 1900

Dihydrodipicolinate Synthase (EC 4.3.3.7; DHDPS), the product of the dapA gene, is an enzyme that catalyzes the condensation of pyruvate and S-aspartate-β-semialdehyde (ASA) into dihydrodipicolinate via an unstable heterocyclic intermediate, (4S)-hydroxy-2,3,4,5-tetrahydro-(2S)-dipicolinic acid. DHDPS catalyzes the first committed step in the biosynthesis of ʟ-lysine and meso-diaminopimelate; each of which is a necessary cross-linking component between peptidoglycan heteropolysacharide chains of bacterial cell walls. Therefore, strong inhibition of DHDPS would result in disruption of meso-diaminopimelate and ʟ-lysine biosynthesis in bacteria leading to decreased bacterial growth and cell lysis. Much attention has been given to targeting the active site for inhibition; however DHDPS is subject to natural feedback inhibition by ʟ-lysine at an allosteric site. In DHDPS from Campylobacter jejuni ʟ-lysine is known to act as a partial uncompetitive inhibitor with respect to pyruvate and a partial mixed inhibitor with respect to ASA. Little is known about how the protein structure facilitates the natural inhibition mechanism and mode of allosteric signal transduction. This work presents ten high resolution crystal structures of Cj-DHDPS and the mutant Y110F-DHDPS with various substrates and inhibitors, including the first reported structure of DHDPS with ASA bound to the active site. As a body of work these structures reveal residues and conformational changes which contribute to the inhibition of the enzyme. Understanding these structure function relationships will be valuable for the design of future antibiotic lead compounds. When an inhibitor binds to the allosteric site there is meaningful shrinkage in the solvent accessible volume between 33% and 49% proportional to the strength of inhibition. Meanwhile at the active site the solvent accessible volume increases between 5% and 35% proportional to the strength of inhibition. Furthermore, inhibitor binding at the allosteric site consistently alters the distance between hydroxyls of the catalytic triad (Y137-T47-Y111') which is likely to affect local pKa's. Changes in active site volume and modification of the catalytic triad would inhibit the enzyme during the binding and condensation of ASA. The residues H56, E88, R60 form a network of hydrogen bonds to close the allosteric site around the inhibitor and act as a lid. Comparison of ʟ-lysine and bislysine bound to wt-DHDPS and Y110F-DHDPS indicates that enhanced inhibition of bislysine is most likely due to increased binding strength rather than altering the mechanism of inhibition. When ASA binds to the active site the network of hydrogen bonds among H56, E88 and R60 is disrupted and the solvent accessible volume of the allosteric site expands by 46%. This observation provides some explanation for the reduced affinity of ʟ-lysine in high ASA concentrations. ʟ-Lysine, but not other inhibitors, is found to induce dynamic domain movements in the wt-DHDPS. These domain movements do not appear to be essential to the inhibition of the enzyme but may play a role in cooperativity between monomers or governing protein dynamics. The moving domain connects the allosteric site to the dimer-dimer interface. Several residues at the weak dimer interface have been identified as potentially involved in dimer-dimer communication including: I172, D173, V176, I194, Y196, S200, N201, K234, D238, Y241, N242 and K245. These residues are not among any previously identified as important for formation of the quaternary structure.

protein crystallography

antibiotic drug design

DHDPS

dihydrodipicolinate synthase

Allostery

Campylobacter jejuni

Étude de la distribution, de la clonalité et caractérisation des campylobacters isolés de poulets à griller et d'humains

Nadeau, Éric

January 2003

Thèse numérisée par la Direction des bibliothèques de l'Université de Montréal.

Campylobacter jejuni

Campylobactériose

Poulet

Humain

Distribution

Risque

Virulence

Gamma-glutamyl transpeptidase

GGT

Detecção dos genes codificantes da toxina CDT e pesquisa de fatores que influenciam a produção de hemolisinas por amostras de Campylobacter jejunide de origem avícola

Trindade, Michele Martins

January 2014

Membros termofílicos do gênero Campylobacter são reconhecidos como importantes enteropatógenos para o ser humano e animais. A grande diversidade ecológica destes microorganismos em diferentes habitats tais como: água, animais e alimentos predispõem ao aparecimento de novos fatores de virulência. Este trabalho teve por objetivo detectar os genes codificantes da Toxina Distensiva Citoletal (CDT) por meio da técnica de PCR, pesquisar a atividade de hemolisinas e a influência de soluções quelantes e de íons nesta atividade. Foram utilizadas 45 amostras de C. jejuni de origem avícolas para pesquisa de atividade hemolítica, cultivadas em Caldo Triptona de Soja (TSB). Após o crescimento bacteriano, as amostras foram semeadas em Ágar tríptico de soja (TSA) contendo 5% de sangue de ovino, equino e bovino, sendo cada sangue testado isoladamente. Para verificar a influência de agentes quelantes e solução de íons na atividade hemolítica, as amostras de C. jejuni foram cultivadas em TSB contendo separadamente os quelantes EDTA, ácido acético, soluções de íons CaCl2 , MgCl2 e FeCl3, em atmosfera de microaerofilia. Quanto à atividade de hemolisina de Campylobacter jejuni em placas de TSA – sangue, foi possível observar que houve hemólises em 48,89% das amostras quando utilizado sangue eqüino, em 40% em sangue de bovino e em 31,11% quando de ovino. Quanto à influência de agentes quelantes e íons em caldo TSB na atividade de hemolisinas em amostras de Campylobacter jejuni semeadas em placas de TSA – sangue ovino, foi observada atividade hemolítica em 26,67% quando utilizado CaCl2, 15,55% (FeCl3), 22,22% (EDTA), 11,11% (MgCl2) e apenas 2,22% (ácido acético). No tocante à atividade hemolítica, o TSA - sangue bovino apresentou 15,55% (CaCl2), 24,44% (FeCl3), 26,26% (EDTA), 20% (MgCl2) e 11,11% (ácido acético). A atividade hemolítica para o sangue equino foi de 24,44% (CaCl2), 22,22% (FeCl3), 28,89% (EDTA), 28,89% (MgCl2) e 8,89% (ácido acético). Para detecção dos genes cdtA, cdtB e cdtC através da técnica da Reação da Polimerase em Cadeia (PCR), foram utilizadas 119 amostras de C. jejuni de origem avícolas. Foi possível observar que 38% possuíam os três genes, e foram identificados somente os genes cdtA e cdtC em 19% do total de amostras, sendo que o gene cdtB foi encontrado em 14%, o gene cdtC foi observado em 12%, os genes cdtA e cdtB em somente 1%, os genes cdtB e cdtC em 1% e para cdtA em 1%. Observou-se que os resultados são dignos de atenção, pois demonstraram em amostras avícolas a presença de estirpes de C. jejuni com potencial virulento. A atividade hemolítica apresentou significativo aumento quando utilizado sangue de origem equina. A mesma foi diminuída quando utilizados agentes quelantes ou íons, nos três tipos de sangue. / Thermophilic members of the Campylobacter genus are recognized as important enteropathogenics for humans and also for other animals. The great diversity of ecological habitats in different organisms such as water, food, and animals may promote new virulence factors. This study aimed at detecting the distending cytolethal toxin (CDT) encoding genes by PCR, studying the activity of hemolysin and also the influence of chelation solutions and ions. A total of 45 samples of C. jejuni from poultry origin, grown in Tryptone Soy Broth (TSB) were used for investigating hemolytic activity. After bacterial growth, samples were plated on Tryptic Soy Agar (TSA) containing 5% sheep, equine or bovine blood, being each blood tested individually. In order to check the influence of chelation agents and ions solution on the hemolytic activity, samples of C. jejuni strains were grown in TSB containing chelation agents individually: EDTA, acetic acid, CaCl2 ion, MgCl2 and FeCl3 solutions, all in microaerophilic atmosphere. Regarding the detection of Campylobacter jejuni hemolysin activity on TSA plates, blood hemolysis were observed in 48.89 % of samples when equine blood was used; in 40% of samples when bovine blood was used and in 31.11 % when the blood used was of sheep origin. The influence of ions and chelation agents in hemolysin activity in TSB when Campylobacter jejuni was plated on TSA with sheep blood can be described as: hemolytic activity was observed at 26.67% of samples when CaCl2 was used, at 15.55 % for FeCl3, 22 22 % for EDTA, 11.11 % for MgCl2 and only 2.22% when acetic acid was used. The hemolytic activity detected when bovine blood - TSA was used indicated 15.55% for CaCl2, 24.44% for FeCl3, 26.26 % for EDTA, 20 % for MgCl2 and 11.11% for acetic acid. In terms of the hemolytic activity when equine blood was used, the results indicated 24.44% for CaCl2, 22.22 % for FeCl3, 28.89 % for EDTA, 28.89 % for MgCl2 and 8.89% for acetic acid. Finally, regarding the detection of cdtA, cdtB and cdtC through PCR, 119 samples of C. jejuni from poultry origin were used. The results indicated that all three genes were present in 38 % of the samples, whereas only two genes were identified in 19 % of samples, while the cdtB gene was singly found in 14%, the cdtC gene was independently observed in 12%, cdtA and cdtB genes together were found in 1% of the samples; the cdtB and cdtC genes associated were detected in 1%, while cdtA alone answered for 1% of detections. The results also showed the presence of C. jejuni strains with virulence potential. The hemolytic activity increased significantly when blood of equine origin was used, and that this activity was reduced when ions or chelating agents were used in combination with the three types of blood cells.

Sanidade avícola

Atividade hemolítica

Aves : Doenças

Campylobacter jejuni

PCR

Hemolytic activity

Ions

Chelants

An epidemiological study of Swedish Campylobacter jejuni isolates from humans and broilers using multilocus sequence typing

Lövström, Tora

January 2009

<p>Campylobacter jejuni is the main cause of bacterial diarrhoeal illness in developed countries, with ~7000 cases being reported each year in Sweden. C. jejuni has received growing attention since it’s recognition as a human pathogen in the 1970s, but its epidemiology is complex and much still remains unknown. There are several potential reservoirs for C. jejuni, including environmental sources as water and soil, wild and domesticated animals, particularly poultry, but also other livestock and pets. In this study 348 Swedish C. jejuni isolates from the year 2000 from humans (n = 164) and broilers (n = 184) were characterized with multilocus sequence typing (MLST) with the aim of comparing the population structures and diversity of C. jejuni between isolates from the two hosts. MLST is a method for characterization of bacterial isolates that indexes the variation in DNA sequence of multiple protein encoding housekeeping genes. A secondary aim in this study was to compare populations of C. jejuni from 11 subgroups of isolates based on location of the sampling. The overlap between the populations was analyzed numerically based on genotypes detected and with analysis of phylogeny, gene flow and molecular variation. It was shown that the population structure of C. jejuni isolates from broilers and humans show a high degree of similarity, supporting broilers as an important source of human infection. However, even though the population structure of human and broiler C. jejuni were almost genetically indistinguishable other sources of C. jejuni infections in humans cannot be ruled out since the same genotypes can be found in other sources as well. Analysis of the 11 subgroups suggested that there may be a difference in populations infecting humans in different Swedish regions, and between populations of C. jejuni in broilers from different slaughterhouses. But this could be a result of chance since most of the subgroups were small. Future studies to improve the understanding of C. jejuni epidemiology, for which MLST has proven itself as a valid method, is important to develop control strategies to prevent infection with this common cause of diarrhoeal illness.</p>

Campylobacter jejuni

multilocus sequence typing

population structure

epidemiology

Outer membrane vesicle-mediated export of virulence factors from Gram-negative bacteria

Rompikuntal, Pramod Kumar

January 2012

The Gram-negative, motile bacterium Campylobacter jejuni is a causative agent of food-borne gastroenteritis. Cytolethal distending toxin (CDT) is one of the important virulence factors for C. jejuni pathogenesis. It was not previously known how CDT is released from C. jejuni into the surrounding environment. In our study, CDT proteins were observed in the periplasmic fraction and all CDT subunits from C. jejuni were released from the bacterial cells in association with OMVs. The OMV-associated toxin caused cytolethal distending effects on tissue culture cells. Our results strongly suggest that the release of OMV-associated CDT is a route by which C. jejuni delivers all CDT toxin subunits (CdtA, CdtB, and CdtC) to the surrounding environment, including infected host tissue.The Gram-negative, motile bacterium Vibrio cholerae is primarily known as the causal organism of the severe dehydrating diarrheal disease cholera. OMVs released from non-O1 non-O139 V. cholerae (NOVC) strain V:5/04 induced an inflammatory response in human host cells. The inflammatory potential is mediated by the nucleotide-binding domain, leucine-rich repeat containing family members NOD1 and NOD2. Physiochemical analysis in conjunction with NOD1/2 reporter assays in HEK293T cells confirmed the presence of the NOD1/2 active peptidoglycan (PGN) in OMVs. Deletion of the quorum sensing master regulator HapR specifically reduced the inflammatory potential of the V:5/04 OMVs and their ability to activate NOD1 and NOD2. These findings suggest that OMVs from a NOVC strain delivered PGN to the host cells, where they elicited an immune response mediated by NOD1 and NOD2.The Gram-negative, non-motile coccobacillus Aggregatibacter actinomycetemcomitans is a natural inhabitant of the oral cavity, but the bacterium can translocate from the oral cavity into the bloodstream and thereby be transported to other regions of the body. A. actinomycetemcomitans is implicated in aggressive forms of periodontitis. The mechanism behind this aggressive periodontitis was not fully known. In addition to several virulence factors, this organism also produces CDT. We have demonstrated that OMVs released by A. actinomycetemcomitans contain several virulence factors, including CDT. We showed that OMVs delivered CDT to the host cells and that CDT was localized inside the nucleus, which led to a cytolethal distending effect on two different cell lines tested: HeLa cells and human gingival fibroblasts (HGF). These results suggest that A. actinomycetemcomitans OMVs could deliver biologically active CDT toxin into the periodontal tissue and may contribute to periodontitis.In our earlier studies, we discovered that an M6 family metalloprotease PrtV was an essential factor for V. cholerae survival from predator grazing. Pure PrtV protein effectively degraded human blood plasma components. In addition, it also showed a dose-dependent cytotoxic effect in the human intestinal HCT8 cell line. V. cholerae produces a large amount of outer membrane vesicles (OMVs) during the normal course of cell growth. OMVs are composed of periplasmic proteins, membrane lipids, lipopolysaccharides and outer membrane proteins. We showed that OMVs can transport several biologically active toxins and enzymes to the surrounding environment and ultimately into the host cells. We have initiated analysis of OMV-associated secretion of virulence factors in V. cholerae. It was observed that PrtV is secreted from V. cholerae wild type strain C6706 into the culture supernatant in association with OMVs and OMV-associated PrtV protein is biologically active and more stable than the free, soluble PrtV protease.

Outer membrane vesicles

CDT

PGN

PrtV

Campylobacter jejuni

Vibrio cholerae

Aggregatibacter actinomycetemcomitans

Identification and characterization of virulence associated factors of C. jejuni

Malik, Abdul

28 October 2010

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Campylobacter jejuni;invasion

formic acid;Motility

42

WF 200: Molekularbiologie

Development of comparative genomic fingerprinting for molecular epidemiological studies of Campylobacter jejuni

Ross, Susan, University of Lethbridge. Faculty of Arts and Science

January 2010

This thesis reports the development of Comparative Genomic Fingerprinting (CGF), a rapid genotyping method for Campylobacter jejuni that assesses the conservation status of 20 genes previously described as having high intraspecies variability based on comparative genomics studies. This novel method for genotyping C. jejuni, CGF was validated two-fold. First, by comparison to flaA restriction fragment length polymorphism analysis, and second a subset of isolates was validated using two higher resolution CGF assays assessing 35 and 119 genes. CGF was then tested in a molecular epidemiological study of C. jejuni isolated from environmental, animal and human clinical samples from southern Alberta. Reservoirs of infection, subtypes associated with higher incidence of human infection, and the persistence of prevalent subtypes in animal/environmental reservoirs were identified. This thesis demonstrates that CGF analysis is robust and can be used to rapidly assess genetic similarity of C. jejuni isolates and to detect epidemiologically relevant clonal groups. / xii, 184 leaves : ill. ; 29 cm

Molecular epidemiology

Dissertations, Academic