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Structural basis for DNA-hairpin promoter recognition by the bacteriophage N4 virion RNA polymerase

机译:噬菌体N4病毒体RNA聚合酶识别DNA发夹启动子的结构基础

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摘要

Coliphage N4 virion-encapsidated RNA polymerase (vRNAP) is a member of the phage T7-like single-subunit RNA polymerase (RNAP) family. Its central domain (mini-vRNAP) contains all RNAP functions of the full-length vRNAP, which recognizes a five- to seven-base pair stem and three-nucleotide loop hairpin DNA promoter. Here we report the X-ray crystal structures of mini-vRNAP bound to promoters. Mini-vRNAP uses four structural motifs to recognize DNA sequences at the hairpin loop and stem, and to unwind DNA. Despite their low sequence similarity, three out of four motifs are shared with T7 RNAP that recognizes a double-stranded DNA promoter. The binary complex structure and results of engineered disulfide-linkage experiments reveal that the plug and motif B loop, which block the access of template DNA to the active site in the apo-form mini-vRNAP, undergo a large-scale conformational change upon promoter binding, explaining the restricted promoter specificity that is critical for N4 phage early transcription.
机译:鹅肠杆菌N4病毒体包裹的RNA聚合酶(vRNAP)是噬菌体T7样单亚基RNA聚合酶(RNAP)家族的成员。它的中央结构域(mini-vRNAP)包含全长vRNAP的所有RNAP功能,该功能可识别5至7个碱基对的茎和3个核苷酸的环状发夹DNA启动子。在这里,我们报告迷你vRNAP绑定到启动子的X射线晶体结构。 Mini-vRNAP使用四个结构基序识别发夹环和茎上的DNA序列,并解开DNA。尽管它们的序列相似性很低,但是与识别双链DNA启动子的T7 RNA共有四个基序。二元复合物的结构和工程化的二硫键连接实验的结果表明,阻止模板DNA进入载脂蛋白型mini-vRNAP中活性位点的塞子和基序B环在启动子上发生了大规模构象变化结合,解释了对N4噬菌体早期转录至关重要的限制性启动子特异性。

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