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在叶绿体mRNA降解过程中,向核酸内切酶切割位点添加富含聚腺苷酸的不稳定序列。

Addition of destabilizing poly (A)-rich sequences to endonuclease cleavage sites during the degradation of chloroplast mRNA.

作者信息

Lisitsky I, Klaff P, Schuster G

机构信息

Department of Biology, Technion-Israel Institute of Technology, Haifa, Israel.

出版信息

Proc Natl Acad Sci U S A. 1996 Nov 12;93(23):13398-403. doi: 10.1073/pnas.93.23.13398.

Abstract

In this work, we report the posttranscriptional addition of poly(A)-rich sequences to mRNA in chloroplasts of higher plants. Several sites in the coding region and the mature end of spinach chloroplast psbA mRNA, which encodes the D1 protein of photosystem II, are detected as polyadenylylated sites. In eukaryotic cells, the addition of multiple adenosine residues to the 3' end of nuclear RNA plays a key role in generating functional mRNAs and in regulating mRNA degradation. In bacteria, the adenylation of several RNAs greatly accelerates their decay. The poly(A) moiety in the chloroplast, in contrast to that in eukaryotic nuclear encoded and bacterial RNAs, is not a ribohomopolymer of adenosine residues, but clusters of adenosines bounded mostly by guanosines and rarely by cytidines and uridines; it may be as long as several hundred nucleotides. Further analysis of the initial steps of chloroplast psbA mRNA decay revealed specific endonuclease cleavage sites that perfectly matched the sites where poly(A)-rich sequences were added. Our results suggest a mechanism for the degradation of psbA mRNA in which endonucleolytic cleavages are followed by the addition of poly(A)-rich sequences to the upstream cleavage products, which target these RNAs for rapid decay.

摘要

在本研究中,我们报道了高等植物叶绿体中mRNA转录后添加富含多聚腺苷酸(poly(A))序列的现象。编码光系统II的D1蛋白的菠菜叶绿体psbA mRNA的编码区和成熟末端的几个位点被检测为多聚腺苷酸化位点。在真核细胞中,向核RNA的3'末端添加多个腺苷残基在产生功能性mRNA和调节mRNA降解中起关键作用。在细菌中,几种RNA的腺苷酸化会极大地加速它们的衰变。与真核细胞核编码的RNA和细菌RNA中的多聚腺苷酸部分不同,叶绿体中的多聚腺苷酸部分不是腺苷残基的核糖同聚物,而是主要由鸟苷包围、很少由胞苷和尿苷包围的腺苷簇;它可能长达数百个核苷酸。对叶绿体psbA mRNA衰变初始步骤的进一步分析揭示了特定的内切核酸酶切割位点,这些位点与添加富含多聚腺苷酸序列的位点完美匹配。我们的结果表明了一种psbA mRNA的降解机制,即内切核酸酶切割后,向上游切割产物添加富含多聚腺苷酸的序列,这些序列将这些RNA靶向快速衰变。

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