Transcriptomic study of 39 ostreid herpesvirus 1 genes during an experimental infection

Massive mortality outbreaks have been reported in France since 2008 among Pacific oysters, Crassostrea gigas, with the detection of a particular OsHV-1 variant called μVar. Virus infection can be induced in healthy spat in experimental conditions allowing to better understand the disease process, in...

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Bibliographic Details
Published in:Journal of Invertebrate Pathology
Main Authors: Segarra, Amelie, Faury, Nicole, Pepin, Jean-francois, Renault, Tristan
Format: Article in Journal/Newspaper
Language:English
Published: Academic Press Inc Elsevier Science 2014
Subjects:
Crassostrea gigas
OsHV-1
Viral gene expression
Inhibitors of apoptosis
Real time PCR
Elongation factor
Pacific
Pacific oyster
Online Access:https://archimer.ifremer.fr/doc/00184/29549/27875.pdf
https://doi.org/10.1016/j.jip.2014.03.002
https://archimer.ifremer.fr/doc/00184/29549/
Description
Summary:Massive mortality outbreaks have been reported in France since 2008 among Pacific oysters, Crassostrea gigas, with the detection of a particular OsHV-1 variant called μVar. Virus infection can be induced in healthy spat in experimental conditions allowing to better understand the disease process, including viral gene expression. Although gene expression of other herpesviruses has been widely studied, we provide the first study following viral gene expression of OsHV-1 over time. In this context, an in vivo transcriptomic study targeting 39 OsHV-1 genes was carried out during an experimental infection of Pacific oyster spat. For the first time, several OsHV-1 mRNAs were detected by real-time PCR at 0 h, 2 h, 4 h, 18 h, 26 h and 42 h post injection. Several transcripts were detected at 2 h post infection and at 18 h post infection for all selected ORFs. Quantification of virus gene expression at different times of infection was also carried out using an oyster housekeeping gene, Elongation factor. Developing an OsHV-1-specific reverse transcriptase real time PCR targeting 39 viral gene appears a new tool in terms of diagnosis and can be used to complement viral DNA detection in order to monitor viral replication.

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