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植物线粒体中编辑位点的识别:5'侧翼序列的重要性

Editing site recognition in plant mitochondria: the importance of 5'-flanking sequences.

作者信息

Williams M A, Kutcher B M, Mulligan R M

机构信息

Department of Developmental and Cell Biology, University of California, Irvine 92697-2300, USA.

出版信息

Plant Mol Biol. 1998 Jan;36(2):229-37. doi: 10.1023/a:1005961718612.

DOI:10.1023/a:1005961718612
PMID:9484435
Abstract

Cytidine to uridine (C-to-U) editing occurs in plant mitochondria with very high specificity such that only specific cytidines are converted to uridines. The mechanisms for editing site selection in plant mitochondria are unknown. In order to examine the determinants of editing site recognition, repeated mitochondrial DNA sequences that include edited nucleotides have been evaluated as editing substrates. During evolution the maize mitochondrial ribosomal protein subunit 12 (rps12) gene recombined with intron 1 of the ribosomal protein subunit 3 (rps3) gene and a region of the S1-like sequence of the 2.3 kb plasmid. These recombinations created a second copy of an internal portion of the rps12 gene, known as rps12b, which includes the first four editing sites of rps12 transcripts. The duplicated sequence extends seven nucleotides upstream of editing site 1 and six nucleotides downstream from editing site 4. The sequences of rps12 and rps12b are identical between these sites except for a single change at -5 from editing site 1. These modifications did not effect C-to-U conversion at editing sites 2, 3, or 4 in rps12b; however, no editing was detected at editing site 1 in rps12b cDNAs. Thus, the 5' recombination abolished editing at site I, while the 3' recombination modified the downstream RNA sequence, but did not effect editing at site IV. Secondary structure prediction suggests that changes in editing site recognition do not correlate with differences in secondary structures, and that primary RNA sequence may be responsible for editing site specification.

摘要

胞苷到尿苷(C 到 U)的编辑在植物线粒体中以非常高的特异性发生,以至于只有特定的胞苷被转化为尿苷。植物线粒体中编辑位点选择的机制尚不清楚。为了研究编辑位点识别的决定因素,包含已编辑核苷酸的重复线粒体 DNA 序列已被评估为编辑底物。在进化过程中,玉米线粒体核糖体蛋白亚基 12(rps12)基因与核糖体蛋白亚基 3(rps3)基因的内含子 1 和 2.3 kb 质粒的 S1 样序列区域发生了重组。这些重组产生了 rps12 基因内部部分的第二个拷贝,称为 rps12b,它包括 rps12 转录本的前四个编辑位点。重复序列在编辑位点 1 上游延伸七个核苷酸,在编辑位点 4 下游延伸六个核苷酸。除了编辑位点 1 上游 -5 处的一个单一变化外,rps12 和 rps12b 在这些位点之间的序列是相同的。这些修饰并未影响 rps12b 中编辑位点 2、3 或 4 的 C 到 U 转化;然而,在 rps12b cDNA 的编辑位点 1 未检测到编辑。因此,5' 重组消除了位点 I 的编辑,而 3' 重组改变了下游 RNA 序列,但不影响位点 IV 的编辑。二级结构预测表明,编辑位点识别的变化与二级结构的差异无关,并且初级 RNA 序列可能负责编辑位点的特异性。

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引用本文的文献

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RNA editing site recognition in heterologous plant mitochondria.异源植物线粒体中的RNA编辑位点识别
Curr Genet. 2006 Dec;50(6):405-16. doi: 10.1007/s00294-006-0100-3. Epub 2006 Oct 11.
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Genetic algorithm learning as a robust approach to RNA editing site prediction.遗传算法学习作为一种预测RNA编辑位点的稳健方法。
BMC Bioinformatics. 2006 Mar 16;7:145. doi: 10.1186/1471-2105-7-145.
3
Different patterns in the recognition of editing sites in plant mitochondria.植物线粒体中编辑位点识别的不同模式。

本文引用的文献

1
RNA editing status of nad7 intron domains in wheat mitochondria.小麦线粒体中nad7内含子结构域的RNA编辑状态
Nucleic Acids Res. 1997 Jan 15;25(2):403-9. doi: 10.1093/nar/25.2.403.
2
Preferential RNA editing at specific sites within transcripts of two plant mitochondrial genes does not depend on transcriptional context or nuclear genotype.两个植物线粒体基因转录本内特定位点的优先RNA编辑不依赖于转录背景或核基因型。
Curr Genet. 1996 Dec;30(6):502-8. doi: 10.1007/s002940050162.
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Sequences directing C to U editing of the plastid psbL mRNA are located within a 22 nucleotide segment spanning the editing site.
Nucleic Acids Res. 2004 Dec 7;32(21):6397-406. doi: 10.1093/nar/gkh969. Print 2004.
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Simple statistical models predict C-to-U edited sites in plant mitochondrial RNA.简单的统计模型可预测植物线粒体RNA中C到U的编辑位点。
BMC Bioinformatics. 2004 Sep 16;5:132. doi: 10.1186/1471-2105-5-132.
5
Electroporation of isolated higher-plant mitochondria: transcripts of an introduced cox2 gene, but not an atp6 gene, are edited in organello.分离的高等植物线粒体的电穿孔:导入的cox2基因的转录本而非atp6基因的转录本在细胞器中被编辑。
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Cross-competition in transgenic chloroplasts expressing single editing sites reveals shared cis elements.在表达单个编辑位点的转基因叶绿体中的交叉竞争揭示了共享的顺式元件。
Mol Cell Biol. 2002 Dec;22(24):8448-56. doi: 10.1128/MCB.22.24.8448-8456.2002.
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cis Recognition elements in plant mitochondrion RNA editing.植物线粒体RNA编辑中的顺式识别元件。
Mol Cell Biol. 2001 Oct;21(20):6731-7. doi: 10.1128/MCB.21.20.6731-6737.2001.
8
Higher plant mitochondria.高等植物线粒体
Plant Cell. 1999 Apr;11(4):571-86. doi: 10.1105/tpc.11.4.571.
引导质体psbL mRNA发生C到U编辑的序列位于跨越编辑位点的一个22个核苷酸的片段内。
EMBO J. 1996 Nov 1;15(21):5958-64.
4
In vivo dissection of cis-acting determinants for plastid RNA editing.质体RNA编辑顺式作用决定因素的体内剖析
EMBO J. 1996 Sep 16;15(18):5052-9.
5
RNA editing: a mechanism for gRNA-specified uridylate insertion into precursor mRNA.RNA编辑:一种将gRNA指定的尿苷酸插入前体mRNA的机制。
Science. 1996 Aug 30;273(5279):1189-95. doi: 10.1126/science.273.5279.1189.
6
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Cell. 1995 Jun 16;81(6):837-40. doi: 10.1016/0092-8674(95)90003-9.