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黏菌绒泡菌同一前体核糖体RNA转录本中的12个I组内含子:RNA加工与进化

Twelve Group I introns in the same pre-rRNA transcript of the myxomycete Fuligo septica: RNA processing and evolution.

作者信息

Lundblad Eirik W, Einvik Christer, Rønning Sissel, Haugli Kari, Johansen Steinar

机构信息

Department of Molecular Biotechnology, RNA research group, Institute of Medical Biology, University of Tromso, Tromso, Norway.

出版信息

Mol Biol Evol. 2004 Jul;21(7):1283-93. doi: 10.1093/molbev/msh126. Epub 2004 Mar 19.

DOI:10.1093/molbev/msh126
PMID:15034133
Abstract

The ribosomal DNA region of the myxomycete Fuligo septica was investigated and found to contain 12 group I introns (four in the small subunit and eight in the large subunit ribosomal RNAs). We have performed molecular and phylogenetic analyses to provide insight into intron structure and function, intron-host biology, and intron origin and evolution. The introns vary in size from 398 to 943 nt, all lacking detectable open reading frames. Secondary structure models revealed considerable structural diversity, but all, except one (subclass IB), represent the common group IC1 intron subclass. In vitro splicing analysis revealed that 10 of the 12 introns were able to self-splice as naked RNA, but all 12 introns were able to splice out from the precursor rRNA in vivo as evaluated by reverse transcription PCR analysis on total F. septica RNA. Furthermore, RNA processing analyses in vitro and in vivo showed that 10 of 12 introns perform hydrolytic cleavage at the 3' splice site, as well as intron circularization. Full-length intron RNA circles were detected in vivo. The order of splicing was analyzed by a reverse transcription PCR approach on cellular RNA, but no strict order of intron excision could be detected. Phylogenetic analysis indicated that most Fuligo introns were distantly related to each other and were independently gained in ribosomal DNA during evolution.

摘要

对黏菌绒泡菌的核糖体DNA区域进行了研究,发现其含有12个I类内含子(小亚基核糖体RNA中有4个,大亚基核糖体RNA中有8个)。我们进行了分子和系统发育分析,以深入了解内含子的结构和功能、内含子与宿主的生物学关系以及内含子的起源和进化。这些内含子大小从398到943个核苷酸不等,均缺乏可检测到的开放阅读框。二级结构模型显示出相当大的结构多样性,但除了一个(IB亚类)之外,所有内含子均代表常见的IC1类内含子亚类。体外剪接分析表明,12个内含子中有10个能够作为裸露RNA进行自我剪接,但通过对绒泡菌总RNA进行逆转录PCR分析评估,所有12个内含子在体内均能从前体rRNA中剪接出来。此外,体外和体内的RNA加工分析表明,12个内含子中有10个在3'剪接位点进行水解切割以及内含子环化。在体内检测到了全长内含子RNA环。通过对细胞RNA进行逆转录PCR方法分析剪接顺序,但未检测到内含子切除的严格顺序。系统发育分析表明,大多数绒泡菌内含子彼此之间关系较远,并且在进化过程中是独立地在核糖体DNA中获得的。

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