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长链双链RNA的解离在体外可通过链置换发生:生物学意义。

Dissociation of long-chain duplex RNA can occur via strand displacement in vitro: biological implications.

作者信息

Homann M, Nedbal W, Sczakiel G

机构信息

Forschungsschwerpunkt Angewandte Tumorvirologie, Deutsches Krebsforschungszentrum, Heidelberg, Germany.

出版信息

Nucleic Acids Res. 1996 Nov 15;24(22):4395-400. doi: 10.1093/nar/24.22.4395.

Abstract

Hammerhead ribozymes with long antisense flanks (>50 bases) have been used successfully to inhibit replication of human immunodeficiency virus type 1 (HIV-1) in living cells. To explain their increased efficacy versus antisense controls or catalytically inactive derivatives, one can consider dissociation of the ribozyme-product complex to allow a complete catalytic cycle. In this work we investigated the dissociation of a double-stranded RNA with 56 bp in vitro. Dissociation was observed in the presence of single-stranded RNA with sequence complementarity to one of the duplex strands. A displacement reaction between RNA single strands and the duplex, but not simple dissociation, was strongly suggested by the concentration dependence of this process, the influence of additional non-complementary sequences on the single strand and by the unusually low Arrhenius activation energy. The strand displacement reaction was slow in vitro at 37 degrees C and physiological ionic strength, but was increased to k approximately 10(3)-10(4)/M/s (approximately 10(4)-fold) at higher temperatures by cetyltrimethylammonium bromide. This compound is thought to enhance non-sequence-specific association of nucleic acids in a mechanistically similar way to that in which cellular hnRNP proteins are thought to act, indicating that strand displacement can be fast and, more importantly, could be tightly regulated in vivo.

摘要

具有长反义侧翼(>50个碱基)的锤头状核酶已成功用于抑制活细胞中1型人类免疫缺陷病毒(HIV-1)的复制。为了解释它们相对于反义对照或催化失活衍生物的疗效增强,人们可以考虑核酶-产物复合物的解离以允许完整的催化循环。在这项工作中,我们在体外研究了一种56 bp双链RNA的解离。在存在与双链体之一具有序列互补性的单链RNA的情况下观察到了解离。RNA单链与双链体之间的置换反应而非简单的解离,由该过程的浓度依赖性、单链上额外非互补序列的影响以及异常低的阿累尼乌斯活化能强烈表明。在37℃和生理离子强度下,体外链置换反应缓慢,但在较高温度下,十六烷基三甲基溴化铵将其提高到k约为10(3)-10(4)/M/s(约10(4)倍)。该化合物被认为以与细胞hnRNP蛋白作用机制相似的方式增强核酸的非序列特异性结合,表明链置换可以很快,更重要的是,在体内可能受到严格调控。

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