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The IE2 regulatory protein of human cytomegalovirus induces expression of the human transforming growth factor beta1 gene through an Egr-1 binding site.

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dc.contributor.authorYoo, YD-
dc.contributor.authorChiou, CJ-
dc.contributor.authorChoi, KS-
dc.contributor.authorYi, Y-
dc.contributor.authorMichelson, S-
dc.contributor.authorKim, S-
dc.contributor.authorHayward, GS-
dc.contributor.authorKim, SJ-
dc.date.accessioned2011-09-27T22:55:49Z-
dc.date.available2011-09-27T22:55:49Z-
dc.date.issued1996-
dc.identifier.issn0022-538X-
dc.identifier.urihttp://repository.ajou.ac.kr/handle/201003/4249-
dc.description.abstractIncreases in transforming growth factor beta1 (TGF-beta1) mRNA and biological activity in the early phase of human cytomegalovirus (CMV) infection in fibroblasts are paralleled by increased TGF-beta1-chloramphenicol acetyltransferase (CAT) reporter gene activity. To determine how CMV infection transactivates the TGF-beta1 promoter, we examined the effects of the cotransfected IE2 regulatory protein of human CMV on 5'-deleted TGF-beta1 promoter-CAT reporter genes in transient DNA transfection assays. Two upstream TGF-beta1 promoter regions each containing an Egr-1 consensus site were shown to be important for IE2-induced transactivation in a cell type that displayed greatly reduced nonspecific activity. Furthermore, transfer of an Egr-l site from between positions -125 and -98, but not point mutant versions of this site, to a heterologous promoter also conveyed IE2 responsiveness. Addition of an IE2 expression vector or use of the U373 A45 astrocytoma cell line expressing IE2 also produced synergistic stimulation of GAL4-Egr-l-mediated activation of a target promoter containing GAL4 binding sites. The 80-kDa IE2 protein present in A45 cells proved to selectively bind to glutathione S-transferase (GST)-Egr-1 beads. The results of in vitro protein binding assays also revealed that an intact in vitro-translated IE2 protein bound directly to the GST-Egr-1 fusion protein through the zinc finger domain of the Egr-1 protein and that this binding activity was abolished by deletion of parts of the zinc finger DNA-binding domain. Similarly, the Egr-1 protein was found to associate preferentially with a small region within the C-terminal half of the IE2 protein adjacent to the DNA-binding and dimerization domains that are important for both transactivation and downregulation. We conclude from these observations that IE2 may regulate transcription of the TGF-beta1 gene as well as other potential cellular targets by virtue of its ability to interact with the Egr-1 DNA-binding protein.-
dc.language.isoen-
dc.subject.MESHAstrocytoma-
dc.subject.MESHCytomegalovirus-
dc.subject.MESHDNA-Binding Proteins-
dc.subject.MESHEarly Growth Response Protein 1-
dc.subject.MESHGene Expression Regulation, Viral-
dc.subject.MESHHumans-
dc.subject.MESHImmediate-Early Proteins-
dc.subject.MESHTranscription Factors-
dc.subject.MESHTranscriptional Activation-
dc.subject.MESHTransforming Growth Factor beta-
dc.subject.MESHTumor Cells, Cultured-
dc.subject.MESHViral Proteins-
dc.titleThe IE2 regulatory protein of human cytomegalovirus induces expression of the human transforming growth factor beta1 gene through an Egr-1 binding site.-
dc.typeArticle-
dc.identifier.pmid8794351-
dc.identifier.urlhttps://www.ncbi.nlm.nih.gov/pmc/articles/PMC190757/-
dc.contributor.affiliatedAuthor최, 경숙-
dc.type.localJournal Papers-
dc.citation.titleJournal of virology-
dc.citation.volume70-
dc.citation.number10-
dc.citation.date1996-
dc.citation.startPage7062-
dc.citation.endPage7070-
dc.identifier.bibliographicCitationJournal of virology, 70(10). : 7062-7070, 1996-
dc.identifier.eissn1098-5514-
dc.relation.journalidJ00022538X-
Appears in Collections:
Journal Papers > School of Medicine / Graduate School of Medicine > Biochemistry & Molecular Biology
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