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由噬菌体T4蛋白产生的复制复合体的结构以及复制叉处的DNA环。

Architecture of the replication complex and DNA loops at the fork generated by the bacteriophage t4 proteins.

作者信息

Chastain Paul D, Makhov Alexander M, Nossal Nancy G, Griffith Jack

机构信息

Lineberger Comprehensive Cancer Center, University of North Carolina, Chapel Hill, North Carolina 27599, USA.

出版信息

J Biol Chem. 2003 Jun 6;278(23):21276-85. doi: 10.1074/jbc.M301573200. Epub 2003 Mar 20.

DOI:10.1074/jbc.M301573200
PMID:12649286
Abstract

Rolling circle replication has previously been reconstituted in vitro using M13 duplex circles containing preformed forks and the 10 purified T4 bacteriophage replication proteins. Leading and lagging strand synthesis in these reactions is coupled and the size of the Okazaki fragments produced is typical of those generated in T4 infections. In this study the structure of the DNAs and DNA-protein complexes engaged in these in vitro reactions has been examined by electron microscopy. Following deproteinization, circular duplex templates with linear tails as great as 100 kb are observed. The tails are fully duplex except for one to three single-stranded DNA segments close to the fork. This pattern reflects Okazaki fragments stopped at different stages in their synthesis. Examination of the DNA-protein complexes in these reactions reveals M13 duplex circles in which 64% contain a single large protein mass (replication complex) and a linear duplex tail. In 56% of the replicating molecules with a tail there is at least one fully duplex loop at the replication complex resulting from the portion of the lagging strand engaged in Okazaki fragment synthesis folding back to the replisome. The single-stranded DNA segments at the fork bound by gene 32 and 59 proteins are not extended but rather appear organized into highly compact structures ("bobbins"). These bobbins constitute a major portion of the mass of the full replication complex.

摘要

滚环复制此前已在体外利用含有预先形成的叉状结构的M13双链环和10种纯化的T4噬菌体复制蛋白得以重建。这些反应中的前导链和滞后链合成是偶联的,所产生的冈崎片段大小与T4感染中产生的片段典型大小相同。在本研究中,通过电子显微镜检查了参与这些体外反应的DNA和DNA-蛋白质复合物的结构。脱蛋白后,观察到具有长达100 kb线性尾巴的环状双链模板。除了靠近叉状结构的一到三个单链DNA片段外,尾巴是完全双链的。这种模式反映了在不同合成阶段停止的冈崎片段。对这些反应中的DNA-蛋白质复合物的检查揭示了M13双链环,其中64%含有单个大的蛋白质团块(复制复合物)和线性双链尾巴。在56%带有尾巴的复制分子中,在复制复合物处至少有一个完全双链环,这是由参与冈崎片段合成的滞后链部分折叠回复制体产生的。由基因32和59蛋白结合的叉状结构处的单链DNA片段没有延伸,而是似乎组织成高度紧凑的结构(“线轴”)。这些线轴构成了完整复制复合物质量的主要部分。

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