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将外切核糖核酸酶 RNase II 和 RNase R 的结构域进行交换:赋予 RNase II 降解双链 RNA 的能力。

Swapping the domains of exoribonucleases RNase II and RNase R: conferring upon RNase II the ability to degrade ds RNA.

机构信息

Instituto de Tecnologia Química e Biológica/Universidade Nova de Lisboa, Apartado 127, 2781-901 Oeiras, Portugal.

出版信息

Proteins. 2011 Jun;79(6):1853-67. doi: 10.1002/prot.23010. Epub 2011 Apr 4.

DOI:10.1002/prot.23010
PMID:21465561
Abstract

RNase II and RNase R are the two E. coli exoribonucleases that belong to the RNase II super family of enzymes. They degrade RNA hydrolytically in the 3' to 5' direction in a processive and sequence independent manner. However, while RNase R is capable of degrading structured RNAs, the RNase II activity is impaired by dsRNAs. The final end-product of these two enzymes is also different, being 4 nt for RNase II and 2 nt for RNase R. RNase II and RNase R share structural properties, including 60% of amino acid sequence similarity and have a similar modular domain organization: two N-terminal cold shock domains (CSD1 and CSD2), one central RNB catalytic domain, and one C-terminal S1 domain. We have constructed hybrid proteins by swapping the domains between RNase II and RNase R to determine which are the responsible for the differences observed between RNase R and RNase II. The results obtained show that the S1 and RNB domains from RNase R in an RNase II context allow the degradation of double-stranded substrates and the appearance of the 2 nt long end-product. Moreover, the degradation of structured RNAs becomes tail-independent when the RNB domain from RNase R is no longer associated with the RNA binding domains (CSD and S1) of the genuine protein. Finally, we show that the RNase R C-terminal Lysine-rich region is involved in the degradation of double-stranded substrates in an RNase II context, probably by unwinding the substrate before it enters into the catalytic cavity.

摘要

RNase II 和 RNase R 是两种属于 RNase II 超家族酶的大肠杆菌外切核酸酶。它们以连续和序列非依赖性的方式从 3'到 5'方向水解 RNA。然而,虽然 RNase R 能够降解结构 RNA,但 RNase II 活性受到双链 RNA 的抑制。这两种酶的最终终产物也不同,RNase II 的终产物是 4 个核苷酸,而 RNase R 的终产物是 2 个核苷酸。RNase II 和 RNase R 具有结构特性,包括 60%的氨基酸序列相似性,并且具有相似的模块化结构域组织:两个 N 端冷休克结构域(CSD1 和 CSD2)、一个中央 RNB 催化结构域和一个 C 端 S1 结构域。我们通过在 RNase II 和 RNase R 之间交换结构域构建了杂交蛋白,以确定哪些结构域负责 RNase R 和 RNase II 之间观察到的差异。结果表明,在 RNase II 背景下,RNase R 的 S1 和 RNB 结构域允许双链底物的降解和 2 个核苷酸长终产物的出现。此外,当 RNase R 的 RNB 结构域不再与真实蛋白的 RNA 结合结构域(CSD 和 S1)相关联时,结构 RNA 的降解变得不依赖于尾部。最后,我们表明,RNase R 的 C 端富含赖氨酸的区域参与了双链底物在 RNase II 背景下的降解,可能是通过在底物进入催化腔之前使其解旋。

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