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Tn7 转座后复合体的结构:一个精心设计的核蛋白结构。

Architecture of the Tn7 posttransposition complex: an elaborate nucleoprotein structure.

机构信息

Howard Hughes Medical Institute, Department of Molecular Biology & Genetics, Johns Hopkins University School of Medicine, 725 North Wolfe Street, 502 PCTB, Baltimore, MD 21205, USA.

出版信息

J Mol Biol. 2010 Aug 13;401(2):167-81. doi: 10.1016/j.jmb.2010.06.003. Epub 2010 Jun 9.

Abstract

Four transposition proteins encoded by the bacterial transposon Tn7, TnsA, TnsB, TnsC, and TnsD, mediate its site- and orientation-specific insertion into the chromosomal site attTn7. To establish which Tns proteins are actually present in the transpososome that executes DNA breakage and joining, we have determined the proteins present in the nucleoprotein product of transposition, the posttransposition complex (PTC), using fluorescently labeled Tns proteins. All four required Tns proteins are present in the PTC in which we also find that the Tn7 ends are paired by protein-protein contacts between Tns proteins bound to the ends. Quantification of the relative amounts of the fluorescent Tns proteins in the PTC indicates that oligomers of TnsA, TnsB, and TnsC mediate Tn7 transposition. High-resolution DNA footprinting of the DNA product of transposition attTn7Colon, two colonsTn7 revealed that about 350 bp of DNA on the transposon ends and on attTn7 contact the Tns proteins. All seven binding sites for TnsB, the component of the transposase that specifically binds the ends and mediates 3' end breakage and joining, are occupied in the PTC. However, the protection pattern of the sites closest to the Tn7 ends in the PTC are different from that observed with TnsB alone, likely reflecting the pairing of the ends and their interaction with the target nucleoprotein complex necessary for activation of the breakage and joining steps. We also observe extensive protection of the attTn7 sequences in the PTC and that alternative DNA structures in substrate attTn7 that are imposed by TnsD are maintained in the PTC.

摘要

细菌转座子 Tn7 编码的 4 种转位蛋白 TnsA、TnsB、TnsC 和 TnsD,介导其在染色体部位 attTn7 处的位点和定向特异性插入。为了确定在执行 DNA 断裂和连接的转座体中实际上存在哪些 Tns 蛋白,我们使用荧光标记的 Tns 蛋白来确定转位后核蛋白产物(后转位复合物,PTC)中存在的蛋白。在 PTC 中存在所有 4 种必需的 Tns 蛋白,我们还发现 Tn7 末端通过结合末端的 Tns 蛋白之间的蛋白-蛋白接触而配对。PTC 中荧光 Tns 蛋白的相对含量的定量表明,TnsA、TnsB 和 TnsC 的寡聚物介导 Tn7 转位。对 attTn7Colon 上 Tn7 转座产物的高分辨率 DNA 足迹分析表明,转座子末端和 attTn7 上约 350bp 的 DNA 与 Tns 蛋白接触。TnsB 是转座酶的组成部分,特异性结合末端并介导 3'末端断裂和连接,它的七个结合位点都被占据在 PTC 中。然而,PTC 中最接近 Tn7 末端的位点的保护模式与单独的 TnsB 观察到的不同,可能反映了末端的配对及其与靶核蛋白复合物的相互作用,这对于激活断裂和连接步骤是必要的。我们还观察到 PTC 中 attTn7 序列的广泛保护,以及 PTC 中由 TnsD 施加的替代 DNA 结构在底物 attTn7 中得以维持。

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