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RNA 结构的柔性区域有助于 Rev 在 Rev 反应元件上进行协同组装。

Flexible regions of RNA structure facilitate co-operative Rev assembly on the Rev-response element.

作者信息

Zemmel R W, Kelley A C, Karn J, Butler P J

机构信息

MRC Laboratory of Molecular Biology, Cambridge, UK.

出版信息

J Mol Biol. 1996 May 24;258(5):763-77. doi: 10.1006/jmbi.1996.0285.

Abstract

The oligomerisation of Rev on the Rev-response element (RRE) was studied using a series of model substrates. Only a monomer of Rev is able to bind efficiently to a high affinity site that is flanked by perfect duplex RNA. Addition of a bulge or a second stem structure adjacent to the high affinity site permits the co-operative incorporation of a second Rev molecule to the RNA. Model RREs carrying bulges can bind Rev with a higher degree of co-operativity than the native structure. Oligomerisation was efficient when the bulge was moved to the opposite strand of the duplex, but was severely impaired when the distance between the bulge and the high affinity site was increased by more than 8 bp. Rev can oligomerise at either end of the RNA-protein complex formed at the high affinity site; when the duplex flanking a high affinity site is disrupted by a bulge or a stem, oligomerisation proceeds in the direction of the disruption regardless of the orientation of the high affinity site. The results are consistent with the "molecular rheostat" model for RRE function, which suggests that Rev binding to the RRE is highly distributive and provides a sensitive measurement of intracellular Rev concentrations.

摘要

利用一系列模型底物研究了Rev在Rev反应元件(RRE)上的寡聚化。只有Rev单体能够有效结合到由完美双链RNA侧翼的高亲和力位点。在高亲和力位点附近添加一个凸起或第二个茎结构可使第二个Rev分子协同掺入到RNA中。带有凸起的模型RREs比天然结构能以更高的协同性结合Rev。当凸起移至双链的相反链时,寡聚化效率较高,但当凸起与高亲和力位点之间的距离增加超过8个碱基对时,寡聚化则严重受损。Rev可在高亲和力位点形成的RNA-蛋白质复合物的任一端进行寡聚化;当高亲和力位点侧翼的双链被凸起或茎破坏时,无论高亲和力位点的方向如何,寡聚化均朝着破坏方向进行。这些结果与RRE功能的“分子变阻器”模型一致,该模型表明Rev与RRE的结合具有高度分布性,并能灵敏地测量细胞内Rev浓度。

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