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通过酵母功能互补克隆的一种编码人CCAAT结合蛋白的cDNA。

A cDNA encoding a human CCAAT-binding protein cloned by functional complementation in yeast.

作者信息

Becker D M, Fikes J D, Guarente L

机构信息

Department of Biology, Massachusetts Institute of Technology, Cambridge 02139.

出版信息

Proc Natl Acad Sci U S A. 1991 Mar 1;88(5):1968-72. doi: 10.1073/pnas.88.5.1968.

Abstract

We constructed a comprehensive cDNA library from HeLa cell mRNA in a vector that directs expression of the cDNA in Saccharomyces cerevisiae. We used this library to clone the human counterpart of the Sa. cerevisiae CCAAT-binding transcription factor, Hap2, by functional complementation of a hap2 mutation. The cDNA encoding the human Hap2 homolog encodes a protein of 257 amino acids that has a 62-amino acid carboxyl-terminal region 73% identical to the essential core region of Hap2. The amino terminus of the protein is highly enriched in glutamine residues, reminiscent of transcriptional activation domains of several other mammalian transcription factors. Analysis of human Hap2 expression reveals three major transcripts: a 4.1-kilobase species found in all cell types examined, a 7.0-kilobase species specific to B lymphocytes, and a 1.6-kilobase species that is expressed preferentially in HeLa cells and that likely corresponds to our cDNA clone. Thus, the human Hap2 homolog and related factors may play both a constitutive and cell type-specific role in gene expression. The general approach of cloning by complementation should allow the isolation of many human genes for which corresponding yeast mutations exist.

摘要

我们以一种能在酿酒酵母中指导cDNA表达的载体,从HeLa细胞mRNA构建了一个全面的cDNA文库。我们利用这个文库,通过对hap2突变进行功能互补,克隆了酿酒酵母CCAAT结合转录因子Hap2的人类对应物。编码人类Hap2同源物的cDNA编码一个257个氨基酸的蛋白质,该蛋白质有一个62个氨基酸的羧基末端区域,与Hap2的必需核心区域有73%的同一性。该蛋白质的氨基末端富含谷氨酰胺残基,这让人联想到其他几种哺乳动物转录因子的转录激活结构域。对人类Hap2表达的分析揭示了三种主要转录本:在所有检测的细胞类型中都存在的一种4.1千碱基的转录本、B淋巴细胞特有的一种7.0千碱基的转录本,以及一种1.6千碱基的转录本,它在HeLa细胞中优先表达,可能与我们的cDNA克隆相对应。因此,人类Hap2同源物及相关因子可能在基因表达中发挥组成性和细胞类型特异性的作用。通过互补进行克隆的一般方法应该能分离出许多存在相应酵母突变的人类基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e820/51147/f01f73e72341/pnas01055-0386-a.jpg

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