2015
DOI: 10.1038/srep18405
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Identification of a highly efficient stationary phase promoter in Bacillus subtilis

Abstract: A promoter that enabled high-level expression of the target gene during the stationary phase in the absence of an inducer would facilitate the efficient production of heterogeneous proteins at a low cost. In this study, a genome-scale microarray-based approach was employed to identify promoters that induced high-level expression of the target genes in Bacillus subtilis from the late log phase to the stationary phase without an inducer. Eleven candidate promoters were selected based on B. subtilis microarray da… Show more

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Cited by 60 publications
(48 citation statements)
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“…The AmyM expression cassette was constructed as follows. Briefly, the promoter P ylb (Yu et al, ), AmyM‐encoding gene amyM containing signal peptide coding sequence (Li et al, ) and T 1 T 2 terminator from pAX01 (Härtl, Wehrl, Wiegert, Homuth, & Schumann, ) were fused by PCR to from AmyM expression cassette. Then, the expression cassette was integrated into the amyE locus through homologous recombination.…”
Section: Methodsmentioning
confidence: 99%
“…The AmyM expression cassette was constructed as follows. Briefly, the promoter P ylb (Yu et al, ), AmyM‐encoding gene amyM containing signal peptide coding sequence (Li et al, ) and T 1 T 2 terminator from pAX01 (Härtl, Wehrl, Wiegert, Homuth, & Schumann, ) were fused by PCR to from AmyM expression cassette. Then, the expression cassette was integrated into the amyE locus through homologous recombination.…”
Section: Methodsmentioning
confidence: 99%
“…The ligation mixture was transformed into E. coli TOP10, and the correct plasmids were identified through colony PCR with corresponding sequencing primers (Additional file 2: Table S2). After confirmation via sequencing, recombinant pUBC19 plasmids were extracted from E. coli TOP10 and transformed into B. subtilis, as described previously [46]. Transformants were harvested by screening the clones on LB agar containing 10 μg/mL kanamycin, and the correct plasmids were verified through colony PCR with the pUBC19 sequencing primers CX-F/CX-R (Additional file 2: Table S2).…”
Section: Construction Of Plasmids For Gene Fragments Heterologous Expmentioning
confidence: 99%
“…The ligation mixture was transformed into E. coli TOP10, and the correct plasmids were identified through colony PCR with corresponding sequencing primers (Table S2). After confirmation via sequencing, recombinant pUBC19 plasmids were extracted from E. coli TOP10 and transformed into B. subtilis, as described previously (Yu, et al 2015). Transformants were harvested by screening the clones on LB agar containing 10 µg/mL kanamycin, and the correct plasmids were verified through colony PCR with the pUBC19 sequencing primers CX-F/CX-R (Table S2).…”
Section: Construction Of Plasmids For Gene Fragments Heterologous Expmentioning
confidence: 99%