Analysis of the P7 region within the catalytic core of the Tetrahymena ribozyme by employing in vitro selection.

Y Oe, Y Ikawa, H Shiraishi, T Inoue
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引用次数: 4

Abstract

The highly conserved P7 region is generally believed to act as a major portion of the catalytic site in the Group I intron ribozyme. However, its functions have not been elucidated except for the fact that it specifically binds a cofactor guanosine required for self-splicing reaction. We attempted an in vitro selection experiment to determine the sequence requirements of this region in the mechanism of catalysis by using the Tetrahymena ribozyme. We found that the selected active clones have the secondary structure similar to that of the wild type with few exceptions. However, their primary sequences were not conserved except G264 and C311 that are the major elements of the binding site for the guanosine. Our results suggest that the unique secondary structure of the P7 region is a primary requisite for the catalytic function of this class of ribozymes.

四膜酶核酶催化核心P7区域的体外筛选分析。
高度保守的P7区域通常被认为是I族内含子核酶催化位点的主要部分。然而,除了特异性结合自剪接反应所需的辅因子鸟苷外,其功能尚未被阐明。我们尝试进行体外选择实验,以确定该区域在四膜虫核酶催化机制中的序列要求。我们发现所选的活性无性系的二级结构与野生型相似,很少有例外。然而,除了鸟苷结合位点的主要元件G264和C311外,它们的初级序列都不保守。我们的研究结果表明,P7区独特的二级结构是这类核酶催化功能的主要必要条件。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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