首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Gene structure for the alpha 1 chain of a human short-chain collagen (type XIII) with alternatively spliced transcripts and translation termination codon at the 5 end of the last exon.
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Gene structure for the alpha 1 chain of a human short-chain collagen (type XIII) with alternatively spliced transcripts and translation termination codon at the 5 end of the last exon.

机译:人类短链胶原蛋白(XIII型)的alpha 1链的基因结构在最后一个外显子的5末端带有交替剪接的转录本和翻译终止密码子。

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摘要

Two overlapping human genomic clones that encode a short-chain collagen, designated alpha 1(XIII), were isolated by using recently described cDNA clones. Characterization of the cosmid clones that span approximately equal to 65,000 base pairs (bp) of the 3' end of the gene established several unusual features of this collagen gene. The last exon encodes solely the 3' untranslated region and it begins with a complete stop codon. The 10 adjacent exons vary in size from 27 to 87 bp and two of them are 54 bp. Therefore, the alpha 1-chain gene of type XIII collagen has some features found in genes for fibrillar collagens but other features that are distinctly different. Previous analysis of overlapping cDNA clones and nuclease S1 mapping of mRNAs indicated one alternative splicing site causing a deletion of 36 bp from the mature mRNA. The present study showed that the 36 bp is contained within the gene as a single exon and also that the gene has a 45-bp -Gly-Xaa-Xaa- repeat coding exon not found in the cDNA clones previously characterized. Nuclease S1 mapping experiments indicated that this 45-bp exon is found in normal human skin fibroblast mRNAs. Accordingly, the data demonstrate that there is alternative splicing of at least two exons of the type alpha 1(XIII)-chain gene.
机译:使用最近描述的cDNA克隆分离了两个重叠的编码短链胶原的人类基因组克隆,称为alpha 1(XIII)。粘粒克隆的特征跨度约等于该基因3'端的65,000个碱基对(bp),建立了该胶原蛋白基因的几个异常特征。最后一个外显子仅编码3'非翻译区,并以完整的终止密码子开始。 10个相邻的外显子大小从27到87 bp不等,其中两个为54 bp。因此,XIII型胶原蛋白的α1链基因具有原纤维胶原蛋白基因中发现的某些特征,但其他特征却明显不同。先前对重叠的cDNA克隆的分析和mRNA的核酸酶S1定位表明,一个可选的剪接位点导致成熟mRNA缺失36 bp。本研究表明该基因包含36 bp作为单个外显子,并且该基因具有45 bp的-Gly-Xaa-Xaa-重复编码外显子,在先前鉴定的cDNA克隆中没有。核酸酶S1作图实验表明,该45-bp外显子存在于正常人皮肤成纤维细胞mRNA中。因此,数据表明存在至少两个α1(XIII)链型外显子的可变剪接。

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