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通过差异噬菌斑滤膜杂交从酿酒酵母中分离半乳糖诱导型DNA序列。

Isolation of galactose-inducible DNA sequences from Saccharomyces cerevisiae by differential plaque filter hybridization.

作者信息

St John T P, Davis R W

出版信息

Cell. 1979 Feb;16(2):443-52. doi: 10.1016/0092-8674(79)90020-5.

DOI:10.1016/0092-8674(79)90020-5
PMID:378392
Abstract

Multiple nitrocellulose DNA filter replicas of plaques of in vitro generated recombinants of phage lambda and Saccharomyces cerevisiae have been screened by hybridization with 32P-labeled cDNA probes. These probes were representative of total poly(A)-containing RNA of yeast cells grown on acetate, galactose, glucose or maltose. This approach allows the use of specific differences in total RNA populations as probes for gene isolation. Five "galactose-induced" clones have been isolated. Expression of the RNA coding regions on at least two cloned sequences, Sc481 and Sc482, is regulated by genes known to control the expression of the structural genes required for the conversion of exogenous galactose to endogenous glucose-1-phosphate. One cloned sequence, Sc484, is expressed during growth on all carbon sources except glucose, and is not under control by the galactose regulatory genes. This clone contains a sequence that is repeated 3 times in the yeast genome. The cloned fragment Sc481 contains coding regions for all or part of three galactose"induced RNAs and may correspond to the GAL 1, GAL 7, GAL 10 gene cluster region of chromosome II.

摘要

通过与32P标记的cDNA探针杂交,对噬菌体λ和酿酒酵母体外产生的重组体噬菌斑的多个硝酸纤维素DNA滤膜复制品进行了筛选。这些探针代表了在乙酸盐、半乳糖、葡萄糖或麦芽糖上生长的酵母细胞中含poly(A)的总RNA。这种方法允许利用总RNA群体中的特定差异作为基因分离的探针。已经分离出五个“半乳糖诱导”克隆。至少两个克隆序列Sc481和Sc482上RNA编码区的表达受已知控制外源半乳糖转化为内源性葡萄糖-1-磷酸所需结构基因表达的基因调控。一个克隆序列Sc484在除葡萄糖外的所有碳源生长过程中表达,且不受半乳糖调节基因的控制。该克隆包含一个在酵母基因组中重复3次的序列。克隆片段Sc481包含三个半乳糖“诱导”RNA全部或部分的编码区,可能对应于第二条染色体的GAL 1、GAL 7、GAL 10基因簇区域。

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