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巨大芽孢杆菌中与钴胺素(维生素B12)生物合成相关的多个基因的克隆

Cloning of multiple genes involved with cobalamin (Vitamin B12) biosynthesis in Bacillus megaterium.

作者信息

Brey R N, Banner C D, Wolf J B

出版信息

J Bacteriol. 1986 Aug;167(2):623-30. doi: 10.1128/jb.167.2.623-630.1986.

Abstract

An effective shotgun cloning procedure was developed for Bacillus megaterium by amplifying gene libraries in Bacillus subtilis. This technique was useful in isolating at least 11 genes from B. megaterium which are involved with cobalamin (vitamin B12) biosynthesis. Amplified plasmid banks were transformed into protoplasts of both a series of Cob mutants blocked before the biosynthesis of cobinamide and Cbl mutants blocked in the conversion of cobinamide into cobalamin. Amplification of gene libraries overcame the cloning barriers inherent in the relatively low protoplast transformation frequency of B. megaterium. A family of plasmids was isolated by complementation of seven different Cob and Cbl mutants. Each plasmid capable of complementing a Cob or Cbl mutant was transformed into each one of the series of Cob and Cbl mutants; many of the plasmids isolated by complementation of one mutation carried genetic activity for complementation of other mutations. By these criteria, four different complementation groups were resolved. At least six genes involved in the biosynthesis of cobinamide are carried on a fragment of DNA approximately 2.7 kilobase pairs in length; other genes involved in the biosynthesis of cobinamide were located in two other complementation groups. The physical and genetic data permitted an ordering of genes within several of the complementation groups. The presence of complementing plasmids in mutants blocked in cobalamin synthesis resulted in restoration of cobalamin biosynthesis.

摘要

通过在枯草芽孢杆菌中扩增基因文库,开发了一种有效的巨大芽孢杆菌鸟枪法克隆程序。该技术有助于从巨大芽孢杆菌中分离出至少11个与钴胺素(维生素B12)生物合成相关的基因。将扩增的质粒文库转化到一系列在钴胺酰胺生物合成之前被阻断的Cob突变体和在钴胺酰胺转化为钴胺素过程中被阻断的Cbl突变体的原生质体中。基因文库的扩增克服了巨大芽孢杆菌原生质体转化频率相对较低所固有的克隆障碍。通过七个不同的Cob和Cbl突变体的互补作用分离出了一个质粒家族。将每个能够互补Cob或Cbl突变体的质粒转化到一系列Cob和Cbl突变体中的每一个中;通过一个突变的互补作用分离出的许多质粒携带了对其他突变进行互补的遗传活性。根据这些标准,解析出了四个不同的互补组。参与钴胺酰胺生物合成的至少六个基因位于一段长度约为2.7千碱基对的DNA片段上;参与钴胺酰胺生物合成的其他基因位于另外两个互补组中。物理和遗传数据允许对几个互补组内的基因进行排序。在钴胺素合成中被阻断的突变体中存在互补质粒导致钴胺素生物合成得以恢复。

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