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ARS Home » Northeast Area » Wyndmoor, Pennsylvania » Eastern Regional Research Center » Molecular Characterization of Foodborne Pathogens Research » Research » Publications at this Location » Publication #301776

Title: Molecular serotyping of Escherichia coli: A verification and reclassification

Author
item Yan, Xianghe
item Fratamico, Pina
item TEBBS, ROBERT - Life Technologies Corporation
item O'CONNELL, CATHERINE - Life Technologies Corporation
item BARANZONI, GIANMARCO - University Of Bologna, Italy
item ALLRED, ADAM - Life Technologies Corporation
item SWIMLEY, MICHELLE - Life Technologies Corporation
item DEBROY, CHOBI - Pennsylvania State University

Submitted to: Meeting Abstract
Publication Type: Abstract Only
Publication Acceptance Date: 2/25/2014
Publication Date: 5/18/2014
Citation: Yan, X., Fratamico, P.M., Tebbs, R., O'Connell, C., Baranzoni, G., Allred, A., Swimley, M., Debroy, C. 2014. Molecular serotyping of Escherichia coli: A verification and reclassification. Meeting Abstract. MA.

Interpretive Summary:

Technical Abstract: Background: Serotyping of E. coli, based on the O- (polysaccharide side chain) and H- (flagellar) antigens using antisera is a common practice for diagnostics, outbreak investigations, and epidemiological surveillance. The full set of E. coli serogroups comprises O-groups O1 to O181, with several O-groups removed. One problem with conventional serotyping is that cross-reactions are observed among different E. coli serogroups, as well as with other bacterial genera. In this study, next generation sequencing technologies were applied to analyze all E. coli O-groups at the genomic level. This work provides information on all of the E. coli O-antigen gene clusters for further investigations and development of molecular serotyping systems, as well as for possible reclassification of E. coli serogroups. Materials and Method: Genomic DNA was isolated from over 75 different E. coli O-group reference strains and subjected to sequencing using the Ion Torrent PGM™. Other O-group sequences were obtained from GenBank. De novo genome assembly of these sequenced strains was performed using CLC Genomics Workbench v 6.5. The entire O-antigen gene cluster was pulled out by alignment with primers that targeted conserved regions in the neighboring JUMPstart region and gnd gene. Nucleotide diversities and species divergence calculations were performed using MEGA 6.0 and clustalW. Results and Conclusion: This is the first comprehensive study of the O-antigen gene clusters from the type strains of all of the known E. coli O-serogroups. Unique sequences within each cluster were identified that will allow for the development of high-throughput molecular serotyping methods and will overcome problems associated with traditional serotyping. The sequence data revealed that some O-groups have very similar O-antigen gene cluster sequences, thus there may be a need to reclassify some E. coli serogroups. This research will enhance the ability of clinical and public health laboratories to serogroup E. coli and may assist in furthering the understanding of the evolution of E. coli.