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大肠杆菌K-12延胡索酸酶基因的克隆、定位与表达

Cloning, mapping, and expression of the fumarase gene of Escherichia coli K-12.

作者信息

Guest J R, Roberts R E

出版信息

J Bacteriol. 1983 Feb;153(2):588-96. doi: 10.1128/jb.153.2.588-596.1983.

Abstract

Two classes of fumarase-transducing phages, lambda fumA and lambda fumB, were isolated from populations of recombinant phages containing HindIII fragments of Escherichia coli DNA; they were isolated by virtue of their ability to complement the metabolic lesion of a fumarase-negative mutant. The strongly complementing lambda fumA phages contained a 6.2-kilobase HindIII fragment encoding: the fumA gene, located at 35.5 min in the E. coli linkage map and expressing the major fumarase activity; the mannosephosphate isomerase gene, manA; and an unidentified gene, g48. The three genes were located relative to the restriction map of the cloned fragment and the genetic linkage map (terC-g48-fumA-manA-uidAoR), their transcription polarities were defined as anticlockwise in the chromosome, and the molecular weights of the corresponding gene products were established: fumA, 61,500; manA, 42,000; g48, 48,000. Organisms containing the fumA gene sub-cloned in multicopy plasmids overproduced fumarase up to 50-fold. The weakly complementing class of transducing phages, lambda fumB, contained several genes in an 8.2-kilobase HindIII fragment, including one (fumB) that determines a minor fumarase activity. Complementation by fumB was only observed in high-copy situations such as transduction plaques and in strains containing a multicopy plasmid in which 40% of normal fumarase activity was detected. The basis for the complementation by fumB was not defined.

摘要

从含有大肠杆菌DNA HindIII片段的重组噬菌体群体中分离出两类转导延胡索酸酶的噬菌体,即λfumA和λfumB;它们是根据其互补延胡索酸酶阴性突变体代谢缺陷的能力而分离得到的。强互补性的λfumA噬菌体含有一个6.2千碱基的HindIII片段,该片段编码:位于大肠杆菌连锁图谱35.5分钟处并表达主要延胡索酸酶活性的fumA基因;磷酸甘露糖异构酶基因manA;以及一个未鉴定的基因g48。这三个基因相对于克隆片段的限制酶切图谱和遗传连锁图谱(terC - g48 - fumA - manA - uidAoR)定位,它们在染色体上的转录极性被确定为逆时针方向,并且确定了相应基因产物的分子量:fumA为61,500;manA为42,000;g48为48,000。含有在多拷贝质粒中亚克隆的fumA基因的生物体过量产生延胡索酸酶,产量高达50倍。弱互补性的转导噬菌体类λfumB在一个8.2千碱基的HindIII片段中含有几个基因,包括一个(fumB)决定次要延胡索酸酶活性的基因。仅在高拷贝情况下,如转导噬菌斑以及含有多拷贝质粒且检测到正常延胡索酸酶活性40%的菌株中观察到fumB的互补作用。fumB互补作用的基础未明确。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a125/221673/ee2aa6039305/jbacter00249-0022-a.jpg

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