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Intramolecular base pairing between the nematode spliced leader and its 5 splice site is not essential for trans-splicing in vitro.

机译：线虫剪接的前导子与其5剪接位点之间的分子内碱基配对对于体外反式剪接不是必需的。

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摘要

The spliced leader RNAs of both trypanosomes and nematodes can form similar secondary structures where the trans-splice donor site is involved in intramolecular base pairing with the spliced leader sequence. It has been proposed that this base pairing could serve to activate autonomously the SL RNA splice donor site. Here, we have examined exon requirements for trans-splicing in a nematode cell free system. Complete disruption of secondary structure interactions at and around the trans-splice donor site did not affect the ability of the SL RNA to function in trans-splicing. In addition, the highly conserved 22 nt sequence could be productively replaced by artificial exons ranging in size from 2 to 246 nucleotides. These results reinforce the view that the 'intron' portion of the SL RNA functions as an independent Sm snRNP whose role is to deliver exon sequences to the trans-spliceosome.

机译：锥虫和线虫的剪接的前导RNA可以形成相似的二级结构，其中跨剪接供体位点与剪接的前导序列与分子内碱基配对。已经提出，该碱基配对可用于自主激活SL RNA剪接供体位点。在这里，我们检查了在无线虫细胞系统中反式剪接的外显子要求。在反剪接供体位点及其周围的二级结构相互作用的完全破坏不影响SL RNA在反剪接中起作用的能力。另外，高度保守的22nt序列可以被大小为2至246个核苷酸的人工外显子有效地替代。这些结果强化了这样一种观点，即SL RNA的“内含子”部分起着独立的Sm snRNP的作用，其作用是将外显子序列传递至反剪接体。

著录项

期刊名称 The EMBO Journal
作者
P A Maroney; G J Hannon; J D Shambaugh; T W Nilsen;
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作者单位

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年(卷),期 1991(10),12
年度 1991
页码 3869–3875
总页数 7
原文格式 PDF
正文语种
中图分类分子生物学;细胞生物学;
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专利

1. Minimum free energy predicted base pairing in the 39 nt spliced leader and 5’ UTR of calmodulin mRNA from Trypanosoma cruzi : influence of the multiple trans-splicing sites [J] . FRANKLYN?SAMUDIO, ADEILTON?BRAND?O Anais da Academia Brasileira de Ciencias . 2018,第2asuppla1期

机译：克氏锥虫钙调蛋白mRNA的39 nt剪接前导序列和5'UTR的最小自由能预测碱基配对：多个反式剪接位点的影响
2. Minimum free energy predicted base pairing in the 39 nt spliced leader and 5 ' UTR of calmodulin mRNA from Trypanosoma cruzi: influence of the multiple trans-splicing sites [J] . Samudio Franklyn, Brandao Adeilton Anais da Academia Brasileira de Ciências . 2018,第1Suppla2期

机译：来自锥虫瘤Cruzi的39 nt拼接前导植物和5'UTR中的最小自由能量预测基础配对和5'UTR的钙调蛋白mRNA：多逆剪接位点的影响
3. Spliced leader trans-splicing in the nematode Trichinella spiralis uses highly polymorphic, noncanonical spliced leaders [J] . Jonathan Pettitt Berndt Müller Ian Stansfield and Bernadette Connolly RNA . 2008,第4期

机译：线虫旋毛虫中的剪接前导反剪使用高度多态的非规范剪接前导
4. Protein Trans-splicing Activities of Multiple Split Inteins Derived from Ssp GyrB Intein [C] . Song Huiling, Meng Qing, Liu Xiang-Qin Biomedical Engineering and Biotechnology (iCBEB), 2012 International Conference on . 2012

机译：来自Ssp GyrB内含子的多个分裂内含子的蛋白质反式分裂活性。
5. Tailoring Big Genes to Small Capsids: Developing Pre-mRNA Trans-splicing Therapies to Treat Genetic Retinal Diseases [D] . Dooley, Scott Joseph. 2018

机译：剪裁大基因到小衣壳：开发前mRNA跨剪接疗法以治疗遗传视网膜疾病
6. Spliced leader trans-splicing in the nematode Trichinella spiralis uses highly polymorphic noncanonical spliced leaders [O] . Jonathan Pettitt, Berndt Müller, Ian Stansfield, 2008

机译：线虫旋毛虫中的剪接前导反剪使用高度多态的非规范剪接前导
7. Intramolecular base pairing between the nematode spliced leader and its 5′ splice site is not essential for trans-splicing in vitro. [O] . P.A. Maroney, G.J. Hannon, J.D. Shambaugh, 1991

机译：线虫剪接领导者和其5'剪接部位之间的分子内碱基对对体外抗碎片不是必需的。

Intramolecular base pairing between the nematode spliced leader and its 5 splice site is not essential for trans-splicing in vitro.

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