Affiliation:
1. Department of Microbiology and Molecular Genetics and Center for the Study of Emerging and Re-emerging Pathogens, University of Texas Medical School, Houston, Texas 77030
Abstract
ABSTRACT
The 5.2-kb ColJs plasmid of a colicinogenic strain of
Shigella sonnei
(colicin type 7) was isolated and sequenced. pColJs was partly homologous to pColE1 and to pesticin-encoding plasmid pPCP1, mainly in the
rep
,
mob
, and
cer
regions. A 1.2-kb unique region of pColJs showed significantly different G+C content (34%) compared to the rest of pColJs (53%). Within the unique region, seven open reading frames (ORFs) were identified. ORF94 was shown to code for colicin Js activity (
cja
), a 94-amino-acid polypeptide (molecular mass, 10.4 kDa); ORF129 (
cji
) was shown to code for the 129-amino-acid colicin Js immunity protein (molecular mass, 14.3 kDa); and ORF65 was shown to be involved in colicin Js release by producer bacteria (
cjl
) coding for a 65-amino-acid polypeptide (molecular mass, 7.5 kDa). In contrast to the gene order in other colicin operons, the
cjl
gene was found upstream from
cja
. Moreover, the promoter upstream from
cjl
was similar to promoters described upstream from several colicin activity genes. The
cji
gene was found to be located downstream from
cja
with a transcription polarity opposite to that of the
cjl
and
cja
genes. The
cja
,
cji
, and
cjl
genes were not similar to other known colicin genes. Colicin Js was purified as an inactive fusion protein with an N-terminal histidine tag. Activity of the purified fusion form of colicin Js was restored after cleavage of the amino acids fused to the colicin Js N terminus.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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