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编码哺乳动物染色体高迁移率族蛋白HMG-I和HMG-Y的mRNA的可变加工

Alternative processing of mRNAs encoding mammalian chromosomal high-mobility-group proteins HMG-I and HMG-Y.

作者信息

Johnson K R, Lehn D A, Reeves R

机构信息

Program in Genetics and Cell Biology Washington State University, Pullman 99164.

出版信息

Mol Cell Biol. 1989 May;9(5):2114-23. doi: 10.1128/mcb.9.5.2114-2123.1989.

Abstract

The high-mobility-group protein HMG-I is a well-characterized nonhistone chromosomal protein that is preferentially expressed in rapidly dividing cells, binds to A. T-rich regions of DNA in vitro, and has been localized to particular regions of mammalian metaphase chromosomes. We isolated eight cDNA clones encoding HMG-I and its isoform HMG-Y from a human Raji cell cDNA library and detected blocks of nucleotide sequence rearrangements in the 5'-untranslated regions of these clones. In addition to this leader sequence variation, five of the eight cDNA clones had either a 33- or 36-base-pair in-frame deletion in their open reading frame (ORF); we found that this shortened ORF encodes the HMG-Y protein isoform. We present evidence that the 5'-untranslated-region and ORF heterogeneity of the cDNA clones is the result of alternative processing of RNA transcripts from a single functional gene. Several additional but probably nonfunctional HMG-I or HMG-Y gene copies exist in the human genome; we isolated and partially sequenced one of these pseudogenes and found that it is a processed HMG-Y retropseudogene.

摘要

高迁移率族蛋白HMG-I是一种特征明确的非组蛋白染色体蛋白,在快速分裂的细胞中优先表达,在体外与富含A.T的DNA区域结合,并已定位到哺乳动物中期染色体的特定区域。我们从人Raji细胞cDNA文库中分离出八个编码HMG-I及其异构体HMG-Y的cDNA克隆,并在这些克隆的5'非翻译区检测到核苷酸序列重排块。除了这种前导序列变异外,八个cDNA克隆中的五个在其开放阅读框(ORF)中具有33或36个碱基对的框内缺失;我们发现这个缩短的ORF编码HMG-Y蛋白异构体。我们提供的证据表明,cDNA克隆的5'非翻译区和ORF异质性是单个功能基因RNA转录本选择性加工的结果。人类基因组中存在几个额外但可能无功能的HMG-I或HMG-Y基因拷贝;我们分离并部分测序了其中一个假基因,发现它是一个加工后的HMG-Y反转录假基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/24d8/363005/a4f15e766284/molcellb00053-0316-a.jpg

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