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酿酒酵母中编码甘氨酸裂解T蛋白的GCV1基因的克隆及分子特征分析

Cloning, and molecular characterization of the GCV1 gene encoding the glycine cleavage T-protein from Saccharomyces cerevisiae.

作者信息

McNeil J B, Zhang F, Taylor B V, Sinclair D A, Pearlman R E, Bognar A L

机构信息

Department of Medical Genetics and Microbiology, University of Toronto, Ont. Canada.

出版信息

Gene. 1997 Feb 20;186(1):13-20. doi: 10.1016/s0378-1119(96)00670-1.

Abstract

We have isolated the gene encoding the glycine cleavage T-protein (GCV1) of the yeast Saccharomyces cerevisiae and shown through gene disruption and enzyme assays that inactivation of GCV1 destroys glycine cleavage function. A DNA fragment encoding the GCV1 gene was cloned by PCR amplification using degenerate oligodeoxyribonucleotides, and the cloned fragment was used as a probe to isolate the complete gene from a yeast genomic library. Growth with glycine stimulated expression of the GCV1 gene as determined by Northern analysis and increased the beta-galactosidase activity of a GCV1-lacZ fusion 30-fold. The URA3 gene was inserted into the coding sequence of GCV1 and the resulting construct was used to disrupt the chromosomal GCV1 gene in a diploid strain of yeast. gcv1::URA3 haploid derivatives grew normally or only slightly more slowly than the isogenic wild-type haploids. All gcv1 strains studied were unable to grow on glycine as a sole nitrogen source and lacked glycine cleavage enzyme activity. Growth of shm1 shm2 mutants was stimulated by glycine, whereas glycine could not supplement the growth of the isogenic gcv1 strain.

摘要

我们已经分离出酿酒酵母甘氨酸裂解T蛋白(GCV1)的编码基因,并通过基因破坏和酶活性测定表明,GCV1失活会破坏甘氨酸裂解功能。使用简并寡脱氧核苷酸通过PCR扩增克隆了编码GCV1基因的DNA片段,并用该克隆片段作为探针从酵母基因组文库中分离出完整基因。通过Northern分析确定,用甘氨酸培养可刺激GCV1基因的表达,并使GCV1 - lacZ融合体的β-半乳糖苷酶活性提高30倍。将URA3基因插入GCV1的编码序列中,并将所得构建体用于破坏酵母二倍体菌株中的染色体GCV1基因。gcv1::URA3单倍体衍生物生长正常,或者仅比同基因野生型单倍体生长略慢。所有研究的gcv1菌株都不能以甘氨酸作为唯一氮源生长,并且缺乏甘氨酸裂解酶活性。shm1 shm2突变体的生长受到甘氨酸的刺激,而甘氨酸不能补充同基因gcv1菌株的生长。

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