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枯草芽孢杆菌模型 RNA 的 5' 端非依赖 RNase J1 内切酶切割。

5' End-independent RNase J1 endonuclease cleavage of Bacillus subtilis model RNA.

机构信息

Department of Pharmacology and Systems Therapeutics, Mount Sinai School of Medicine, New York, New York 10029-6574, USA.

出版信息

J Biol Chem. 2011 Oct 7;286(40):34932-40. doi: 10.1074/jbc.M111.287409. Epub 2011 Aug 23.

Abstract

Bacillus subtilis trp leader RNA is a small (140-nucleotide) RNA that results from attenuation of trp operon transcription upon binding of the regulatory TRAP complex. Previously, endonucleolytic cleavage by ribonuclease RNase J1 in a 3'-proximal, single-stranded region was shown to be critical for initiation of trp leader RNA decay. RNase J1 is a dual-specificity enzyme, with both 5' exonucleolytic and endonucleolytic activities. Here, we provide in vivo and in vitro evidence that RNase J1 accesses its internal target site on trp leader RNA in a 5' end-independent manner. This has important implications for the role of RNase J1 in RNA decay. We also tested the involvement in trp leader RNA decay of the more recently discovered endonuclease RNase Y. Half-lives of several trp leader RNA constructs, which were designed to probe pathways of endonucleolytic versus exonucleolytic decay, were measured in an RNase Y-deficient mutant. Remarkably, the half-lives of these constructs were indistinguishable from their half-lives in an RNase J1-deficient mutant. These results suggest that lowering RNase Y concentration may affect RNA decay indirectly via an effect on RNase J1, which is thought to exist with RNase Y in a degradosome complex. To generalize our findings with trp leader RNA to other RNAs, we show that the mechanism of trp leader RNA decay is not dependent on TRAP binding.

摘要

枯草芽孢杆菌 trp 启动子 RNA 是一种小的(140 个核苷酸)RNA,它是在结合调节性 TRAP 复合物后,trp 操纵子转录衰减的结果。以前的研究表明,核糖核酸酶 RNase J1 在 3'近端的单链区域进行内切核酸酶切割,对于 trp 启动子 RNA 衰变的起始至关重要。RNase J1 是一种双特异性酶,具有 5'外切核酸酶和内切核酸酶活性。在这里,我们提供了体内和体外证据,证明 RNase J1 以 5'端非依赖的方式进入其在 trp 启动子 RNA 上的内部靶位点。这对 RNase J1 在 RNA 衰变中的作用具有重要意义。我们还测试了最近发现的内切核酸酶 RNase Y 是否参与 trp 启动子 RNA 衰变。在 RNase Y 缺陷突变体中,测量了几种 trp 启动子 RNA 构建体的半衰期,这些构建体旨在探测内切核酸酶与外切核酸酶衰变的途径。值得注意的是,这些构建体的半衰期与它们在 RNase J1 缺陷突变体中的半衰期相同。这些结果表明,降低 RNase Y 浓度可能会通过对 RNase J1 的间接影响来影响 RNA 衰变,RNase J1 被认为与 RNase Y 存在于降解体复合物中。为了将我们在 trp 启动子 RNA 上的发现推广到其他 RNA,我们表明 trp 启动子 RNA 衰变的机制不依赖于 TRAP 结合。

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