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Development of a new host vector system in mycobacteria.

作者信息

Goto Y, Taniguchi H, Udou T, Mizuguchi Y, Tokunaga T

机构信息

Faculty of Agriculture, Miyazaki University, Japan.

出版信息

FEMS Microbiol Lett. 1991 Oct 15;67(3):277-82. doi: 10.1016/0378-1097(91)90489-w.

Abstract

The hybrid plasmid pYT72/pYT92 constructed from an Escherichia coli plasmid pACYC177 and mycobacterial plasmid pMSC262 isolated from Mycobacterium scroflaceum strain W262 transformed both E. coli and BCG. Phage-sensitive mutants S-10 and S-20 isolated from BCG Tokyo strain showed higher frequency of transformation than the wild-type strain. Frequency of transformation was dependent on age of the culture and the electroporation condition used. Several deletion mutants were generated from pYT72/92 to determine the minimum region for the replication in the mycobacteria. A 2.3-kb fragment of pMSC262 was found to contain an essential region. Using this fragment and pACYC177, a small shuttle vector pYT937 containing two drug-resistance markers, kanamycin- and ampicillin-resistance, was constructed. pYT937 contains AatII, BamHI, BbvII, GsuI, HincII, PstI, ScaI and XbaI cloning sites.

摘要

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