Detection of recombinant breakpoint in the genome of human enterovirus E11 strain associated with a fatal nosocomial outbreak

Martina Rueca; Simone Lanini; Emanuela Giombini; Francesco Messina; Concetta Castilletti; Giuseppe Ippolito; Maria Rosaria Capobianchi; Maria Beatrice Valli

doi:10.1186/s12985-022-01821-2

Detection of recombinant breakpoint in the genome of human enterovirus E11 strain associated with a fatal nosocomial outbreak

Virol J. 2022 Jun 3;19(1):97. doi: 10.1186/s12985-022-01821-2.

Authors

Martina Rueca¹, Simone Lanini¹, Emanuela Giombini², Francesco Messina¹, Concetta Castilletti¹, Giuseppe Ippolito¹, Maria Rosaria Capobianchi¹, Maria Beatrice Valli¹

Affiliations

¹ National Institute for Infectious Diseases L. Spallanzani IRCCS, Rome, Italy.
² National Institute for Infectious Diseases L. Spallanzani IRCCS, Rome, Italy. emanuela.giombini@inmi.it.

Abstract

Background: The aim of this study was to characterize the genome of a recombinant Enterovirus associated with severe and fatal nosocomial infection; it was typed as Echovirus 11 (E-11) according to the VP1 gene. Enterovirus infection is generally asymptomatic and self-limited, but occasionally it may progress to a more severe clinical manifestation, as in the case described here. Recombination plays a crucial role in the evolution of Enteroviruses (EVs) and has been recognized as the main driving force behind the emergence of epidemic strains associated with severe infection. Therefore, it is of utmost importance to monitor the circulation of recombinant strains for surveillance purposes.

Methods: Enterovirus-RNA was detected in the serum and liver biopsy of patients involved in the nosocomial cluster by commercial One-Step qRT-PCR method and the Enterovirus strains were isolated in vitro. The EVs typing was determined by analyzing the partial-length of the 5'UTR and VP1 sequences with the web-based open-access Enterovirus Genotyping Tool Version 0.1. The amplicons targeting 5'UTR, VP1 and overlapping fragments of the entire genome were sequenced with the Sanger method. Phylogenetic analysis was performed comparing the VP1 and the full-genome sequences of our strains against an appropriate reference set of Enterovirus prototypes of the Picornaviridae genera and species retrieved from the Enterovirus Genotyping Tool. Recombination analysis was performed using RDP4 software.

Results: The Neighbor-Joining tree of the VP1 gene revealed that the 4 patients were infected with an identical molecular variant of Echovirus 11 (E-11). While the phylogenetic and the RDP4 analysis of the full-genome sequences provided evidence that it was a chimeric strain between an E-11 and a Coxsackievirus B (CV-B).

Conclusions: The chimeric structure of the E-11 genome might have contributed to the severe infection and epidemic feature of the strain, but further biological characterizations are needed. The evidence reported in this study, highlights the limit of typing techniques based on the VP1 gene, as they fail to identify the emergence of recombinant strains with potentially more pathogenic or epidemic properties, thus providing only partial information on the epidemiology and pathogenesis of Enteroviruses.

Keywords: Enterovirus; Phylogeny; Recombination.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

5' Untranslated Regions
Cross Infection* / epidemiology
Disease Outbreaks
Enterovirus B, Human
Enterovirus Infections* / epidemiology
Enterovirus*
Genome, Viral
Humans
Phylogeny
RNA, Viral / chemistry
RNA, Viral / genetics

Substances

5' Untranslated Regions
RNA, Viral