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STRUCTURE OF THE UMUD' PROTEIN AND ITS REGULATION IN RESPONSE TO DNA DAMAGE

机译:UMUD蛋白质的结构及其对DNA损伤的响应调控

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摘要

FOR life to be sustained, mistakes in DNA repair must be tolerated when damage obscures the genetic information. In bacteria such as Escherichia coli, DNA damage elicits the well regulated 'SOS response' (reviewed in ref. 1). For the extreme case of damage that cannot be repaired by conventional enzymes, there are proteins that allow the replication of DNA through such lesions, but with a reduction in the fidelity of replication(2). Essential proteins in this mutagenic process are RecA, DNA polymerase III, UmuD, UmuD' and UmuC (umu: UV mutagenesis)(1-3). Regulation of this response involves a RecA-mediated self-cleavage of UmuD to produce UmuD'. To understand this system in more detail, we have determined the crystal structure of the E. coli UmuD' mutagenesis protein at 2.5 Angstrom resolution. Globular heads folded in an unusual beta-structure associate to form molecular dimers, and extended amino-terminal tails associate to produce crystallized filaments. The structure provides insight into the mechanism of the self-cleavage reaction that UmuD-like proteins undergo as part of the global SOS response(4-8). [References: 30]
机译:为了维持生命,当损害掩盖了遗传信息时,必须容忍DNA修复中的错误。在诸如大肠杆菌的细菌中,DNA损伤引发了良好调节的“ SOS反应”(参见参考文献1)。对于无法用常规酶修复的极端损伤,有些蛋白质可以使DNA通过此类损伤进行复制,但复制的保真度会降低(2)。在该诱变过程中,必需蛋白是RecA,DNA聚合酶III,UmuD,UmuD'和UmuC(umu:UV诱变)(1-3)。该反应的调节涉及RemuA介导的UmuD自我切割以产生UmuD'。为了更详细地了解此系统,我们确定了2.5埃分辨率的大肠杆菌UmuD'诱变蛋白的晶体结构。球状头折叠成不寻常的β结构,缔合形成分子二聚体,延伸的氨基末端尾形缔合,产生结晶长丝。该结构提供了对UmuD样蛋白作为整体SOS响应一部分进行的自我切割反应机理的洞察力(4-8)。 [参考:30]

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