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布氏锥虫布鲁斯亚种四个小核U RNA基因的分离与测序:U2、U4和U6 RNA类似物的鉴定

Isolation and sequence of four small nuclear U RNA genes of Trypanosoma brucei subsp. brucei: identification of the U2, U4, and U6 RNA analogs.

作者信息

Mottram J, Perry K L, Lizardi P M, Lührmann R, Agabian N, Nelson R G

机构信息

University of California Intercampus Program in Molecular Parasitology, Schools of Pharmacy, San Francisco.

出版信息

Mol Cell Biol. 1989 Mar;9(3):1212-23. doi: 10.1128/mcb.9.3.1212-1223.1989.

Abstract

Trypanosomes use trans splicing to place a common 39-nucleotide spliced-leader sequence on the 5' ends of all of their mRNAs. To identify likely participants in this reaction, we used antiserum directed against the characteristic U RNA 2,2,7-trimethylguanosine (TMG) cap to immunoprecipitate six candidate U RNAs from total trypanosome RNA. Genomic Southern analysis using oligonucleotide probes constructed from partial RNA sequence indicated that the four largest RNAs (A through D) are encoded by single-copy genes that are not closely linked to one another. We have cloned and sequenced these genes, mapped the 5' ends of the encoded RNAs, and identified three of the RNAs as the trypanosome U2, U4, and U6 analogs by virtue of their sequences and structural homologies with the corresponding metazoan U RNAs. The fourth RNA, RNA B (144 nucleotides), was not sufficiently similar to known U RNAs to allow us to propose an identify. Surprisingly, none of these U RNAs contained the consensus Sm antigen-binding site, a feature totally conserved among several classes of U RNAs, including U2 and U4. Similarly, the sequence of the U2 RNA region shown to be involved in pre-mRNA branchpoint recognition in yeast, and exactly conserved in metazoan U2 RNAs, was totally divergent in trypanosomes. Like all other U6 RNAs, trypanosome U6 did not contain a TMG cap and was immunoprecipitated from deproteinized RNA by anti-TMG antibody because of its association with the TMG-capped U4 RNA. These two RNAs contained extensive regions of sequence complementarity which phylogenetically support the secondary-structure model proposed by D. A. Brow and C. Guthrie (Nature [London] 334:213-218, 1988) for the organization of the analogous yeast U4-U6 complex.

摘要

锥虫利用反式剪接将一个共同的39个核苷酸的剪接前导序列置于其所有mRNA的5'端。为了鉴定该反应中可能的参与成分,我们使用针对特征性U RNA 2,2,7-三甲基鸟苷(TMG)帽的抗血清,从锥虫总RNA中免疫沉淀六种候选U RNA。使用根据部分RNA序列构建的寡核苷酸探针进行的基因组Southern分析表明,四个最大的RNA(A至D)由单拷贝基因编码,这些基因彼此之间没有紧密连锁。我们已经克隆并测序了这些基因,绘制了编码RNA的5'端图谱,并通过与相应后生动物U RNA的序列和结构同源性,将其中三个RNA鉴定为锥虫U2、U4和U6类似物。第四个RNA,RNA B(144个核苷酸),与已知的U RNA相似性不足,无法让我们提出其身份。令人惊讶的是,这些U RNA中没有一个包含共有Sm抗原结合位点,这是在包括U2和U4在内的几类U RNA中完全保守的特征。同样,在酵母中显示参与前体mRNA分支点识别且在后生动物U2 RNA中完全保守的U2 RNA区域序列,在锥虫中完全不同。与所有其他U6 RNA一样,锥虫U6不包含TMG帽,并且由于其与TMG加帽的U4 RNA相关联,可通过抗TMG抗体从脱蛋白RNA中免疫沉淀。这两个RNA包含广泛的序列互补区域,从系统发育角度支持了D. A. Brow和C. Guthrie(《自然》[伦敦]334:213 - 218, 1988)提出的类似酵母U4 - U6复合物组织的二级结构模型。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c589/362712/379c66e10b46/molcellb00051-0348-a.jpg

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