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Nuclear Mutants of Maize with Defects in Chloroplast Polysome Assembly Have Altered Chloroplast RNA Metabolism.叶绿体多核糖体组装存在缺陷的玉米核突变体具有改变的叶绿体RNA代谢。
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Recruitment of a peptidyl-tRNA hydrolase as a facilitator of group II intron splicing in chloroplasts.招募一种肽基-tRNA水解酶作为叶绿体中II类内含子剪接的促进因子。
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The bI4 group I intron binds directly to both its protein splicing partners, a tRNA synthetase and maturase, to facilitate RNA splicing activity.BI4 组 I 内含子直接与其两种蛋白质剪接伙伴(一种 tRNA 合成酶和成熟酶)结合,以促进 RNA 剪接活性。
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Predicting subcellular localization of proteins based on their N-terminal amino acid sequence.基于蛋白质N端氨基酸序列预测其亚细胞定位
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Sequence-specific RNA binding by a Nova KH domain: implications for paraneoplastic disease and the fragile X syndrome.Nova KH 结构域对序列特异性 RNA 的结合:对副肿瘤性疾病和脆性 X 综合征的影响。
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10
A reverse transcriptase/maturase promotes splicing by binding at its own coding segment in a group II intron RNA.逆转录酶/成熟酶通过结合II组内含子RNA中其自身的编码区段来促进剪接。
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CRS1是一种新型的II类内含子剪接因子,它起源于一个古老的结构域。

CRS1 is a novel group II intron splicing factor that was derived from a domain of ancient origin.

作者信息

Till B, Schmitz-Linneweber C, Williams-Carrier R, Barkan A

机构信息

Institute of Molecular Biology, University of Oregon, Eugene 97403, USA.

出版信息

RNA. 2001 Sep;7(9):1227-38. doi: 10.1017/s1355838201010445.

DOI:10.1017/s1355838201010445
PMID:11565746
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1370168/
Abstract

Protein-dependent group II intron splicing provides a forum for exploring the roles of proteins in facilitating RNA-catalyzed reactions. The maize nuclear gene crs1 is required for the splicing of the group II intron in the chloroplast atpF gene. Here we report the molecular cloning of the crs1 gene and an initial biochemical characterization of its gene product. Several observations support the notion that CRS1 is a bona fide group II intron splicing factor. First, CRS1 is found in a ribonucleoprotein complex in the chloroplast, and cofractionation data provide evidence that this complex includes atpF intron RNA. Second, CRS1 is highly basic and includes a repeated domain with features suggestive of a novel RNA-binding domain. This domain is related to a conserved free-standing open reading frame of unknown function found in both the eubacteria and archaea. crs1 is the founding member of a gene family in plants that was derived by duplication and divergence of this primitive gene. In addition to its previously established role in atpF intron splicing, new genetic data implicate crs1 in chloroplast translation. The chloroplast splicing and translation functions of crs1 may be mediated by the distinct protein products of two crs1 mRNA forms that result from alternative splicing of the crs1 pre-mRNA.

摘要

蛋白质依赖性II类内含子剪接为探索蛋白质在促进RNA催化反应中的作用提供了一个平台。玉米核基因crs1是叶绿体atpF基因中II类内含子剪接所必需的。在此,我们报告crs1基因的分子克隆及其基因产物的初步生化特性。多项观察结果支持CRS1是一种真正的II类内含子剪接因子这一观点。首先,CRS1存在于叶绿体中的核糖核蛋白复合物中,共分级分离数据表明该复合物包含atpF内含子RNA。其次,CRS1具有高度碱性,包含一个重复结构域,其特征表明它是一个新的RNA结合结构域。该结构域与在真细菌和古细菌中发现的功能未知的保守独立开放阅读框相关。crs1是植物中一个基因家族的创始成员,该家族由这个原始基因的复制和分化而来。除了其先前确定的在atpF内含子剪接中的作用外,新的遗传数据表明crs1参与叶绿体翻译。crs1的叶绿体剪接和翻译功能可能由crs1前体mRNA可变剪接产生的两种crs1 mRNA形式的不同蛋白质产物介导。