噬菌体T4中双链断裂刺激的依赖重组的DNA复制。
Recombination-dependent DNA replication stimulated by double-strand breaks in bacteriophage T4.
作者信息
Kreuzer K N, Saunders M, Weislo L J, Kreuzer H W
机构信息
Department of Microbiology, Duke University Medical Center, Durham, North Carolina 27710, USA.
出版信息
J Bacteriol. 1995 Dec;177(23):6844-53. doi: 10.1128/jb.177.23.6844-6853.1995.
We analyzed the mechanism of recombination-dependent DNA replication in bacteriophage T4-infected Escherichia coli using plasmids that have sequence homology to the infecting phage chromosome. Consistent with prior studies, a pBR322 plasmid, initially resident in the infected host cell, does not replicate following infection by T4. However, the resident plasmid can be induced to replicate when an integrated copy of pBR322 vector is present in the phage chromosome. As expected for recombination-dependent DNA replication, the induced replication of pBR322 required the phage-encoded UvsY protein. Therefore, recombination-dependent plasmid replication requires homology between the plasmid and phage genomes but does not depend on the presence of any particular T4 DNA sequence on the test plasmid. We next asked whether T4 recombination-dependent DNA replication can be triggered by a double-strand break (dsb). For these experiments, we generated a novel phage strain that cleaves its own genome within the nonessential frd gene by means of the I-TevI endonuclease (encoded within the intron of the wild-type td gene). The dsb within the phage chromosome substantially increased the replication of plasmids that carry T4 inserts homologous to the region of the dsb (the plasmids are not themselves cleaved by the endonuclease). The dsb stimulated replication when the plasmid was homologous to either or both sides of the break but did not stimulate the replication of plasmids with homology to distant regions of the phage chromosome. As expected for recombination-dependent replication, plasmid replication triggered by dsbs was dependent on T4-encoded recombination proteins. These results confirm two important predictions of the model for T4-encoded recombination-dependent DNA replication proposed by Gisela Mosig (p. 120-130, in C. K. Mathews, E. M. Kutter, G. Mosig, and P. B. Berget (ed.), Bacteriophage T4, 1983). In addition, replication stimulated by dsbs provides a site-specific version of the process, which should be very useful for mechanistic studies.
我们使用与感染噬菌体染色体具有序列同源性的质粒,分析了噬菌体T4感染的大肠杆菌中依赖重组的DNA复制机制。与先前的研究一致,最初存在于受感染宿主细胞中的pBR322质粒在T4感染后不会复制。然而,当噬菌体染色体中存在pBR322载体的整合拷贝时,驻留质粒可以被诱导复制。正如依赖重组的DNA复制所预期的那样,pBR322的诱导复制需要噬菌体编码的UvsY蛋白。因此,依赖重组的质粒复制需要质粒和噬菌体基因组之间的同源性,但不依赖于测试质粒上任何特定T4 DNA序列的存在。接下来,我们询问T4依赖重组的DNA复制是否可以由双链断裂(dsb)触发。对于这些实验,我们构建了一种新型噬菌体菌株,该菌株通过I-TevI核酸内切酶(编码在野生型td基因的内含子中)在非必需的frd基因内切割其自身基因组。噬菌体染色体内的dsb显著增加了携带与dsb区域同源的T4插入片段的质粒的复制(这些质粒本身不会被核酸内切酶切割)。当质粒与断裂的一侧或两侧同源时,dsb会刺激复制,但不会刺激与噬菌体染色体远处区域同源的质粒的复制。正如依赖重组的复制所预期的那样,由dsb触发的质粒复制依赖于T4编码的重组蛋白。这些结果证实了Gisela Mosig提出的T4编码的依赖重组的DNA复制模型的两个重要预测(见C.K.Mathews、E.M.Kutter、G.Mosig和P.B.Berget(编),《噬菌体T4》,1983年,第120 - 130页)。此外,由dsb刺激的复制提供了该过程的位点特异性版本,这对于机制研究应该非常有用。
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