来自乳酸乳球菌噬菌体phi31的噬菌体诱导型中间启动子及其转录激活因子的分子特征
Molecular characterization of a phage-inducible middle promoter and its transcriptional activator from the lactococcal bacteriophage phi31.
作者信息
Walker S A, Klaenhammer T R
机构信息
Department of Food Science, Southeast Dairy Foods Research Center, North Carolina State University, Raleigh 27695-7624, USA.
出版信息
J Bacteriol. 1998 Feb;180(4):921-31. doi: 10.1128/JB.180.4.921-931.1998.
An inducible middle promoter from the lactococcal bacteriophage phi31 was isolated previously by shotgun cloning an 888-bp fragment (P15A10) upstream of the beta-galactosidase (beta-Gal) gene (lacZ.st) from Streptococcus thermophilus (D. J. O'Sullivan, S. A. Walker, S. G. West, and T. R. Klaenhammer, Bio/Technology 14:82-87, 1996). The promoter showed low levels of constitutive beta-Gal activity which could be induced two- to threefold over baseline levels after phage infection. During this study, the fragment was subcloned and characterized to identify a smaller, tightly regulated promoter fragment which allowed no beta-Gal activity until after phage infection. This fragment, defined within nucleotides 566 to 888 (P(566-888); also called fragment 566-888), contained tandem, phage-inducible transcription start sites at nucleotides 703 and 744 (703/744 start sites). Consensus -10 regions were present upstream of both start sites, but no consensus -35 regions were identified for either start site. A transcriptional activator, encoded by an open reading frame (ORF2) upstream of the 703/744 start sites, was identified for P(566-888). ORF2 activated P(566-888) when provided in trans in Escherichia coli. In addition, when combined with pTRK391 (P15A10::lacZ.st) in Lactococcus lactis NCK203, an antisense ORF2 construct was able to retard induction of the phage-inducible promoter as measured by beta-Gal activity levels. Finally, gel shift assays showed that ORF2 was able to bind to promoter fragment 566-888. Deletion analysis of the region upstream from the tandem promoters identified a possible binding site for transcriptional activation of the phage promoters. The DNA-binding ability of ORF2 was eliminated upon deletion of part of this region, which lies centered approximately 35 bp upstream of start site 703. Deletion analysis and mutagenesis studies also elucidated a critical region downstream of the 703/744 start sites, where mutagenesis resulted in a two- to threefold increase in beta-Gal activity. With these improvements, the level of expression achieved by an explosive-expression strategy was elevated from 3,000 to 11,000 beta-Gal units within 120 min after induction.
先前通过鸟枪法克隆嗜热链球菌β-半乳糖苷酶(β-Gal)基因(lacZ.st)上游的一个888 bp片段(P15A10),分离出了来自乳球菌噬菌体phi31的一个可诱导中间启动子(D. J. 奥沙利文、S. A. 沃克、S. G. 韦斯特和T. R. 克莱恩哈默,《生物技术》14:82 - 87,1996年)。该启动子显示出低水平的组成型β-Gal活性,在噬菌体感染后可诱导至比基线水平高两到三倍。在本研究中,对该片段进行了亚克隆和表征,以鉴定一个更小、调控严格的启动子片段,该片段在噬菌体感染前不具有β-Gal活性。这个在核苷酸566至888范围内定义的片段(P(566 - 888);也称为片段566 - 888),在核苷酸703和744处含有串联的、噬菌体诱导的转录起始位点(703/744起始位点)。两个起始位点上游均存在一致的 -10区域,但未鉴定到任一起始位点的一致 -35区域。鉴定出一个由703/744起始位点上游的一个开放阅读框(ORF2)编码的转录激活因子,用于P(566 - 888)。当在大肠杆菌中反式提供时,ORF2激活P(566 - 888)。此外,当与乳酸乳球菌NCK203中的pTRK391(P15A10::lacZ.st)组合时,一个反义ORF2构建体能够通过β-Gal活性水平来延缓噬菌体诱导型启动子的诱导。最后,凝胶迁移试验表明ORF2能够结合启动子片段566 - 888。对串联启动子上游区域的缺失分析鉴定出一个可能用于噬菌体启动子转录激活的结合位点。删除该区域中位于起始位点703上游约35 bp中心位置的部分后,ORF2的DNA结合能力丧失。缺失分析和诱变研究还阐明了703/744起始位点下游的一个关键区域,诱变导致该区域的β-Gal活性增加两到三倍。通过这些改进,在诱导后120分钟内,通过爆发性表达策略实现的表达水平从3000个β-Gal单位提高到了11000个β-Gal单位。
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