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人端粒酶RNA野生型假结的溶液结构与动力学

Solution structure and dynamics of the wild-type pseudoknot of human telomerase RNA.

作者信息

Kim Nak-Kyoon, Zhang Qi, Zhou Jing, Theimer Carla A, Peterson Robert D, Feigon Juli

机构信息

Department of Chemistry and Biochemistry, P.O. Box 951569, University of California, Los Angeles, CA 90095-1569, USA.

出版信息

J Mol Biol. 2008 Dec 31;384(5):1249-61. doi: 10.1016/j.jmb.2008.10.005. Epub 2008 Oct 11.

Abstract

Telomerase is a ribonucleoprotein complex that replicates the 3' ends of linear chromosomes by successive additions of telomere repeat DNA. The telomerase holoenzyme contains two essential components for catalysis, a telomerase reverse transcriptase (TERT) and telomerase RNA (TER). The TER includes a template for telomere repeat synthesis as well as other domains required for function. We report the solution structure of the wild-type minimal conserved human TER pseudoknot refined with an extensive set of RDCs, and a detailed analysis of the effect of the bulge U177 on pseudoknot structure, dynamics analyzed by RDC and 13C relaxation measurements, and base pair stability. The overall structure of PKWT is highly similar to the previously reported DeltaU177 pseudoknot (PKDU) that has a deletion of a conserved bulge U important for catalytic activity. For direct comparison to PKWT, the structure of PKDU was re-refined with a comparable set of RDCs. Both pseudoknots contain a catalytically essential triple helix at the junction of the two stems, including two stem 1-loop 2 minor groove triples, a junction loop 1-loop 2 Hoogsteen base pair, and stem 2-loop 1 major groove U.A-U Watson-Crick-Hoogsteen triples located directly above the bulge U177. However, there are significant differences in the stabilities of base pairs near the bulge and the dynamics of some nucleotides. The stability of the base pairs in stem 2 surrounding the bulge U177 is greatly decreased, with the result that the Watson-Crick pairs in the triple helix begin to unfold before the Hoogsteen pairs, which may affect telomerase assembly and activity. The bulge U is positioned in the minor groove on the face opposite the triple helical interactions, and sterically blocks the A176 2'OH, which has recently been proposed to have a role in catalysis. The bulge U may serve as a hinge providing backbone flexibility in this region.

摘要

端粒酶是一种核糖核蛋白复合体,通过连续添加端粒重复DNA来复制线性染色体的3'末端。端粒酶全酶包含两个催化必需的组分,即端粒酶逆转录酶(TERT)和端粒酶RNA(TER)。TER包括端粒重复序列合成的模板以及功能所需的其他结构域。我们报道了野生型最小保守人类TER假结的溶液结构,该结构通过大量剩余偶极耦合(RDC)进行了精修,并对凸起U177对假结结构、通过RDC和13C弛豫测量分析的动力学以及碱基对稳定性的影响进行了详细分析。PKWT的整体结构与先前报道的DeltaU177假结(PKDU)高度相似,后者缺失了对催化活性很重要的保守凸起U。为了与PKWT进行直接比较,PKDU的结构用一组可比的RDC进行了重新精修。两个假结在两个茎的交界处都包含一个催化必需的三螺旋,包括两个茎1-环2小沟三联体、一个连接环1-环2 Hoogsteen碱基对以及位于凸起U177正上方的茎2-环1大沟U·A-U沃森-克里克-Hoogsteen三联体。然而,凸起附近碱基对的稳定性以及一些核苷酸的动力学存在显著差异。围绕凸起U177的茎2中碱基对的稳定性大大降低,结果三螺旋中的沃森-克里克对在Hoogsteen对之前开始展开,这可能会影响端粒酶的组装和活性。凸起U位于与三螺旋相互作用相对的面上的小沟中,空间上阻碍了最近被认为在催化中起作用的A176 2'OH。凸起U可能充当一个铰链,在该区域提供主链灵活性。

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