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大肠杆菌中核糖醇和D-阿拉伯糖醇分解代谢的基因:它们在C菌株中的位点以及在K-12和B菌株中的缺失。

Genes for ribitol and D-arabitol catabolism in Escherichia coli: their loci in C strains and absence in K-12 and B strains.

作者信息

Reiner A M

出版信息

J Bacteriol. 1975 Aug;123(2):530-6. doi: 10.1128/jb.123.2.530-536.1975.

Abstract

Escherichia coli C strains can grow at the expense of the two natural pentitols ribitol and D-arabitol, sugar alcohols previously thought not to be utilized by E. coli. E. coli strains K-12 and B cannot utilize either compound. The genetic loci responsible for pentitol catabolism in E. coli C, designated rtl and atl, are separate and closely linked. Each lies between metG and his and is highly co-transducible with metG and with a P2 prophage attachment site. rtl and atl readily can be transduced into E. coli K-12 or B strains, in which they integrate at, or very near, their E. coli C location. Transduction also can be used to insert rtl and atl into certain E. coli K-12 F' plasmids. No recombination between E. coli C strains and either K-12 or B strains occurs within the rtl-atl genetic region after interstrain conjugations or transductions. No cryptic rtl or atl genes in K-12 or B strains can be detected by complementation, recombination, or mutagenesis. These results are consistent with the view that the rtl-atl portion of the E. coli C chromosome has no counterpart in E. coli K-12 or B and may have been obtained from an extrageneric source. Detailed biochemical and genetic comparisons of penitol utilization in E. coli and Klebsiella aerogenes are in progress. The ability to catabolize xylitol is conferred upon E. coli C strains by a mutation at or adjacent to the rtl locus, whereas in E. coli K-12 or B strains harboring rtl an additional mutation at a separate locus is required for xylitol utilization.

摘要

大肠杆菌C菌株能够利用两种天然戊糖醇——核糖醇和D -阿拉伯糖醇进行生长,而这两种糖醇此前被认为不能被大肠杆菌利用。大肠杆菌K - 12和B菌株均不能利用这两种化合物。在大肠杆菌C中负责戊糖醇分解代谢的基因位点,分别命名为rtl和atl,它们是分开的但紧密连锁。每个位点都位于metG和his之间,并且与metG以及一个P2原噬菌体附着位点具有高度共转导性。rtl和atl很容易被转导到大肠杆菌K - 12或B菌株中,它们在其中整合到与大肠杆菌C中的位置相同或非常接近的位置。转导也可用于将rtl和atl插入某些大肠杆菌K - 12 F'质粒中。在菌株间进行接合或转导后,大肠杆菌C菌株与K - 12或B菌株在rtl - atl基因区域内不会发生重组。通过互补、重组或诱变,在K - 12或B菌株中检测不到隐藏的rtl或atl基因。这些结果与以下观点一致:大肠杆菌C染色体的rtl - atl部分在大肠杆菌K - 12或B中没有对应物,可能是从非同源来源获得的。目前正在对大肠杆菌和产气克雷伯菌中戊糖醇利用进行详细的生化和遗传比较。木糖醇分解代谢能力是由rtl位点或其附近的一个突变赋予大肠杆菌C菌株的,而在携带rtl的大肠杆菌K - 12或B菌株中,木糖醇利用还需要在一个单独位点发生额外突变。

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