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首页> 外文期刊>The Journal of biological chemistry >Structural basis of RNA polymerase recycling by the Swi2/Snf2 family of ATPase RapA in Escherichia coli
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Structural basis of RNA polymerase recycling by the Swi2/Snf2 family of ATPase RapA in Escherichia coli

机译:SWI2 / SNF2 ATPASE RAPA在大肠杆菌中RNA聚合酶的结构基础

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After transcription termination, cellular RNA polymerases (RNAPs) are occasionally trapped on DNA, impounded in an undefined post-termination complex (PTC), limiting the free RNAP pool and subsequently leading to inefficient transcription. In Escherichia coli, a Swi2/Snf2 family of ATPase called RapA is known to be involved in countering such inefficiency through RNAP recycling; however, the precise mechanism of this recycling is unclear. To better understand its mechanism, here we determined the structures of two sets of E. coli RapA–RNAP complexes, along with the RNAP core enzyme and the elongation complex, using cryo-EM. These structures revealed the large conformational changes of RNAP and RapA upon their association that has been implicated in the hindrance of PTC formation. Our results along with DNA-binding assays reveal that although RapA binds RNAP away from the DNA-binding main channel, its binding can allosterically close the RNAP clamp, thereby preventing its nonspecific DNA binding and PTC formation. Taken together, we propose that RapA acts as a guardian of RNAP by which RapA prevents nonspecific DNA binding of RNAP without affecting the binding of promoter DNA recognition σ factor, thereby enhancing RNAP recycling.
机译:在转录终止之后,细胞RNA聚合酶(RNAAP)偶尔被困在DNA上,在未定义的终止后络合物(PTC)中扣押,限制了游离的RNAP池并随后导致效率低下的转录。在大肠杆菌中,已知称为RAPA的SWI2 / SNF2家族ATP酶是通过RNAP回收来反击这种效率;然而,这种回收的确切机制尚不清楚。为了更好地理解其机制,在这里,我们确定了两组大肠杆菌RAN-RNAP复合物的结构,以及使用CREYO-EM的RNAP核心酶和伸长型复合物。这些结构揭示了rnap和Rapa在其关联中的大构象变化,这与PTC形成的障碍有关。我们的结果随着DNA结合测定结果表明,尽管RAPA结合RNAP远离DNA结合主通道,但其结合可以构成rNAP钳位,从而防止其非特异性DNA结合和PTC形成。我们建议,RAPA作为RNAP的监护人,RNA可防止RNAP的非特异性DNA结合而不影响启动子DNA识别σ因子的结合,从而提高RNAP再循环。

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