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dc.contributor.authorDizman, Yeşim Aktürk
dc.contributor.authorDemirbağ, Zihni
dc.contributor.authorİnce, İkbal Agah
dc.contributor.authorNalcacıoğu, Remziye
dc.date.accessioned2020-12-19T20:05:14Z
dc.date.available2020-12-19T20:05:14Z
dc.date.issued2012
dc.identifier.citationDizman, YA., Demirbağ, Z., İnce, IA., Nalçacıoğlu, R. (2012). Transcriptomic analysis of Chilo iridescent virus immediate early promoter. Virus Research, 167(2), 353-357.en_US
dc.identifier.issn0168-1702
dc.identifier.issn1872-7492
dc.identifier.urihttps://doi.org/10.1016/j.virusres.2012.05.025
dc.identifier.urihttps://hdl.handle.net/11436/3421
dc.descriptionDemirbag, Zihni/0000-0001-5487-1977; INCE, Ikbal Agah/0000-0003-2299-9946; Nalcacioglu, Remziye/0000-0003-0527-9541en_US
dc.descriptionWOS: 000306889100027en_US
dc.descriptionPubMed: 22698875en_US
dc.description.abstractChilo iridescent virus (CIV) is an insect virus belonging to the Iridoviridae. the DNA genome (212,482 base pairs) is entirely sequenced, however very little is known about viral gene regulation, expression and function. the structure and transcriptional regulation of the CIV 012L gene is investigated in this study. Infection of Bombyx mori SPC-BM-36 cells in the presence of Ara-C (inhibits DNA replication) or cycloheximide (inhibits protein synthesis), followed by RT-PCR on isolated total RNA, showed that CIV 012L is transcribed as an immediate-early gene. Detecting the RNA transcript of the CIV 012L early in infection confirmed the data about the temporal class of the gene obtained with the inhibitors. Time course transcription of the gene showed that the transcription starts immediately after infection and reach up to maximum level at 4 h p.i. 5' RACE analysis on RNA isolated from CIV-infected BM cells showed that the transcription initiation site is located 30 nucleotides upstream of the translational start codon. To map the limits of the putative promoter of this gene, upstream sequences of various lengths were cloned in front of a firefly luciferase reporter gene. the resulting plasmid constructs were tested in a transfection assay, in which the baculovirus IE-1 promoter fused to Renilla luciferase was used as an internal control for transfection efficiency. A gradual reduction in luciferase expression occurred as the deletions extended from -200 to -10, relative to the transcription start site. It is clearly shown that sequences between -20 and -10 relative to the transcription start site have key promoter activity for CIV 012L gene. However this key sequence could not be found at the upstream region of CIV's other potential immediate early genes. (c) 2012 Elsevier B.V. All rights reserved.en_US
dc.description.sponsorshipScientific and Technological Research Council of Turkey, TUBITAKTurkiye Bilimsel ve Teknolojik Arastirma Kurumu (TUBITAK) [107T916]en_US
dc.description.sponsorshipThis work was supported by the Scientific and Technological Research Council of Turkey, TUBITAK with Project No: 107T916.en_US
dc.language.isoengen_US
dc.publisherElsevier Science Bven_US
dc.rightsinfo:eu-repo/semantics/closedAccessen_US
dc.subjectChilo iridescent virusen_US
dc.subjectCIV 012Len_US
dc.subjectImmediate-earlyen_US
dc.subjectPromoter analysisen_US
dc.subjectTranscriptome analysisen_US
dc.titleTranscriptomic analysis of Chilo iridescent virus immediate early promoteren_US
dc.typearticleen_US
dc.contributor.departmentRTEÜ, Fen - Edebiyat Fakültesi, Biyoloji Bölümüen_US
dc.contributor.institutionauthorDizman, Yeşim Aktürk
dc.identifier.doi10.1016/j.virusres.2012.05.025
dc.identifier.volume167en_US
dc.identifier.issue2en_US
dc.identifier.startpage353en_US
dc.identifier.endpage357en_US
dc.relation.journalVirus Researchen_US
dc.relation.publicationcategoryMakale - Uluslararası Hakemli Dergi - Kurum Öğretim Elemanıen_US


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