Please use this identifier to cite or link to this item: https://ninho.inca.gov.br/jspui/handle/123456789/6901
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dc.contributor.authorBrant, Ayslan Castro-
dc.contributor.authorMajerciak, Vladimir-
dc.contributor.authorMoreira, Miguel Angelo Martins-
dc.contributor.authorZheng, Zhi-Ming-
dc.date.accessioned2022-05-11T19:01:17Z-
dc.date.available2022-05-11T19:01:17Z-
dc.date.issued2019-
dc.identifier.issn1995-820X-
dc.identifier.other10.1007/s12250-019-00098-0-
dc.identifier.urihttp://sr-vmlxaph03:8080/jspui/handle/123456789/6901-
dc.description.abstractHuman papillomavirus 18 (HPV18) E6 and E7 oncogenes are transcribed as a single bicistronic E6E7 pre-mRNA. The E6 ORF region in the bicistronic E6E7 pre-mRNA contains an intron. Splicing of this intron disrupts the E6 ORF integrity and produces a spliced E6*I RNA for efficient E7 translation. Here we report that the E6 intron has two overlapped branch point sequences (BPS) upstream of its 3' splice site, with an identical heptamer AACUAAC, for E6*I splicing. One heptamer has a branch site adenosine (underlined) at nt 384 and the other at nt 388. E6*I splicing efficiency correlates to the expression level of E6 and E7 proteins and depends on the selection of which branch site. In general, E6*I splicing prefers the 3'ss-proximal branch site at nt 388 over the distal branch site at nt 384. Inactivation of the nt 388 branch site was found to activate a cryptic acceptor site at nt 636 for aberrant RNA splicing. Together, these data suggest that HPV18 modulates its production ratio of E6 and E7 proteins by alternative selection of the two mapped branch sites for the E6*I splicing, which could be beneficial in its productive or oncogenic infection according to the host cell environment.pt_BR
dc.language.isoenpt_BR
dc.publisherVirologica Sinicapt_BR
dc.subjectHuman papillomavirus 18pt_BR
dc.subjectPapillomavirus Humano 18pt_BR
dc.subjectHPV-18pt_BR
dc.subjectPapillomavirus E7 Proteinspt_BR
dc.subjectProteínas E7 de Papillomaviruspt_BR
dc.subject.otherHPV Splicingen
dc.titleHPV18 Utilizes Two Alternative Branch Sites for E6*I Splicing to Produce E7 Proteinpt_BR
dc.TypeArticlept_BR
Appears in Collections:Artigos de Periódicos da Pesquisa Experimental e Translacional

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