Control of expression by the cellulose synthase ( bcsA) promoter region from Acetobacter xylinum BPR 2001
The 5′ upstream region (about 3.1 kb) of the cellulose synthase operon ( bcs operon) has been isolated by cloning from Acetobacter xylinum strain BPR 2001. The expression level of the upstream region was determined using sucrose synthase cDNA as a reporter gene in the shuttle vector pSA19. The expre...
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Veröffentlicht in: | Gene 1998-06, Vol.213 (1), p.93-100 |
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Sprache: | eng |
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Zusammenfassung: | The 5′ upstream region (about 3.1
kb) of the cellulose synthase operon (
bcs operon) has been isolated by cloning from
Acetobacter xylinum strain BPR 2001. The expression level of the upstream region was determined using sucrose synthase cDNA as a reporter gene in the shuttle vector pSA19. The expression occurred with the 1.1-kb upstream sequence from the ATG start codon of the
bcs operon but not with the 241-bp upstream sequence in
A. xylinum, although neither the 1.1-kb nor the 241-bp upstream sequence caused any expression as a promoter in
Escherichia coli. The level of expression with the 1.1-kb upstream sequence in
A. aceti was 75% of that in
A. xylinum. These results suggest that the upstream region functions as a specific promoter for the
Acetobacter genus. The expression was reduced by the introduction of the 241-bp upstream region between the
lac promoter and the reporter gene in
E. coli and was not detected in
A. xylinum. This suggests that the short upstream region composed of 241
bp contains the site(s) which causes a negative regulation on the transcription for
bcs operon. The production of recombinant protein with the ribosome-binding site (RBS) of
A. xylinum obtained from the
bcs operon, was reduced to about half in
E. coli, and that with the site of the
lac promoter was also reduced to about half in
A. xylinum. This shows that a species-specific predominance occurs during interaction between mRNA and 16S rRNA in the RBS between
A. xylinum and
E. coli. |
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ISSN: | 0378-1119 1879-0038 |
DOI: | 10.1016/S0378-1119(98)00191-7 |