home > bioproject > PRJEB3017
identifier PRJEB3017
type bioproject
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organism
title Anguillid herpesvirus 1 cDNA library deep sequencing
description We used deep sequencing of poly(A) RNA to characterize the transcriptome of an economically important eel herpesvirus, anguillid herpesvirus 1 (AngHV1), at a stage during the lytic life cycle when infectious virus was being produced. In contrast to mammalian herpesviruses, the overall level of antisense transcription from the 248526 bp genome was low, amounting to only 1.5% of transcription in predicted protein-coding regions, and no abundant, nonoverlapping, noncoding RNAs were identified. RNA splicing was found to be more common than had been anticipated previously. Counting the 10634 bp terminal direct repeat once, 100 splice junctions were identified, of which 58 were inferred to be the most likely to be functional because they represent splicing between protein-coding exons or between 5-untranslated regions and protein-coding exons. Each of the 30 most highly represented of the 58 splice junctions was confirmed by RT-PCR. We also used deep sequencing to identify numerous putative 5- and 3-ends of AngHV1 transcripts, confirming some of these and adding others by RACE. The findings prompted a revision of the AngHV1 genome map to include a total of 129 protein-coding genes, five of which are duplicated in the terminal direct repeat. Eleven genes contain integral, spliced protein-coding exons, and nine contain 5-untranslated exons or, because of alternative splicing, 5-untranslated and 5-translated exons. The results of this study sharpen our understanding of AngHV1 genomics, and provide the first detailed view of a fish herpesvirus transcriptome.
data type Other
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publication
properties 
{...}
dbXrefs
sra-run  ERR125657ERR125658
sra-submission  ERA129522ERA129523
biosample  SAMEA1325054SAMEA1325053
sra-study  ERP001424
sra-sample  ERS138736ERS138737
sra-experiment  ERX101814ERX101815
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status public
visibility unrestricted-access
dateCreated 2012-05-22T01:00:00Z
dateModified 2012-05-22T01:00:00Z
datePublished 2012-05-22T01:00:00Z