Pederson N E, Person S, Homa F L
Department of Molecular and Cell Biology, Pennsylvania State University, University Park 16802.
J Virol. 1992 Oct;66(10):6226-32. doi: 10.1128/JVI.66.10.6226-6232.1992.
To investigate the cis-acting sequences involved in regulation of a herpes simplex virus gamma 1 gene, deletion analyses of the glycoprotein B (gB) gene promoter were performed. In transfection assays with gB-chloramphenicol acetyltransferase plasmids, high-level constitutive expression from the gB promoter was found with an 89-bp sequence (-69 to +20). Additional sequences in the 5'-transcribed noncoding leader region (+20 to +136) were required for full stimulation by herpes simplex virus infection. Plasmids with progressive deletions of the gB leader sequence demonstrated that chloramphenicol acetyltransferase expression in infected cells was proportional to the length of the leader region retained. In recombinant viruses containing a gB-gC gene fusion, a similar 83-bp (-60 to +23) region of the gB gene was found to promote accurately initiated gC mRNA from the viral genome with the same kinetics as the wild-type gB gene. Although the kinetics of expression remained the same, RNA abundance was greater with a 298-bp (-260 to +38) promoter than with the 83-bp promoter.
为了研究单纯疱疹病毒γ1基因调控中涉及的顺式作用序列,对糖蛋白B(gB)基因启动子进行了缺失分析。在用gB-氯霉素乙酰转移酶质粒进行的转染试验中,发现gB启动子的一个89bp序列(-69至+20)可实现高水平的组成型表达。单纯疱疹病毒感染进行完全刺激需要5'-转录非编码前导区(+20至+136)中的其他序列。带有gB前导序列逐步缺失的质粒表明,感染细胞中氯霉素乙酰转移酶的表达与保留的前导区长度成正比。在含有gB-gC基因融合的重组病毒中,发现gB基因的一个类似的83bp(-60至+23)区域能以与野生型gB基因相同的动力学从病毒基因组中准确起始gC mRNA。尽管表达动力学保持不变,但298bp(-260至+38)启动子的RNA丰度高于83bp启动子。
