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一种增强IE-1反式激活的39K基因表达的苜蓿银纹夜蛾核多角体病毒立即早期基因的功能图谱分析

Functional mapping of an AcNPV immediately early gene which augments expression of the IE-1 trans-activated 39K gene.

作者信息

Carson D D, Guarino L A, Summers M D

机构信息

Department of Biochemistry and Biophysics, Texas A&M University, College Station.

出版信息

Virology. 1988 Feb;162(2):444-51. doi: 10.1016/0042-6822(88)90485-0.

Abstract

An early gene which augments the expression of the delayed early/late 39K gene of the baculovirus Autographa californica nuclear polyhedrosis virus (AcNPV) was identified by functional mapping. Transient expression of the plasmid p39CAT, containing the bacterial chloramphenicol acetyltransferase coding sequences under the control of the promoter of the 39K protein, was observed in cells cotransfected with AcNPV DNA digested with several restriction endonucleases. However, when p39CAT was cotransfected with viral DNA digested with Bg/II restriction endonuclease, no CAT activity could be detected. To map the location of the Bg/II-sensitive sequences required for efficient expression of 39CAT, p39CAT and Bg/II-digested viral DNA were cotransfected with a PstI library of AcNPV DNA. The PstI-N fragment restored 39CAT activity. A major early 1.3-kb transcript from this fragment was mapped by S1 nuclease analysis. Transient assay experiments indicated that this major transcript of the PstI-N fragment was produced by an immediate early gene, named IE-N. The PstI-N fragment alone did not activate expression of p39CAT but was required when IE-1 was present in limiting quantities.

摘要

通过功能图谱分析鉴定出一种早期基因,该基因可增强杆状病毒苜蓿银纹夜蛾核型多角体病毒(AcNPV)延迟早期/晚期39K基因的表达。在用几种限制性内切酶消化的AcNPV DNA共转染的细胞中,观察到质粒p39CAT的瞬时表达,该质粒含有在39K蛋白启动子控制下的细菌氯霉素乙酰转移酶编码序列。然而,当p39CAT与用Bg/II限制性内切酶消化的病毒DNA共转染时,未检测到CAT活性。为了定位有效表达39CAT所需的Bg/II敏感序列的位置,将p39CAT和Bg/II消化的病毒DNA与AcNPV DNA的PstI文库共转染。PstI-N片段恢复了39CAT活性。通过S1核酸酶分析确定了该片段的一个主要早期1.3kb转录本。瞬时分析实验表明,PstI-N片段的这个主要转录本由一个立即早期基因产生,命名为IE-N。单独的PstI-N片段不会激活p39CAT的表达,但当IE-1的量有限时是必需的。

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