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Novel sinIR promoter for Bacillus subtilis DB104 recombinant protein expression systemopen access

Authors
Jun, Ji-SuKim, Min-JooHong, KwangWon
Issue Date
Mar-2023
Publisher
한국응용생명화학회
Keywords
Bacillus subtilis DB104; Expression system; Promoter engineering; sinIR promoter
Citation
Journal of Applied Biological Chemistry, v.66, pp 128 - 137
Pages
10
Indexed
SCOPUS
KCI
Journal Title
Journal of Applied Biological Chemistry
Volume
66
Start Page
128
End Page
137
URI
https://scholarworks.dongguk.edu/handle/sw.dongguk/20580
DOI
10.3839/jabc.2023.019
ISSN
1976-0442
2234-7941
Abstract
Transcriptome analysis revealed that the sinR gene encoding a transition-state regulator of Bacillus pumilus, genetically close to B. subtilis, was expressed at high levels during growth. The sinR gene is the second gene of the sinIR operon consisting of three promoters and two structural genes in B. subtilis. This study used the sinIR promoter of B. subtilis DB104 to construct a recombinant protein expression system. First, the expression ability depending on the number of sinIR promoter was investigated using enhanced green fluorescent protein (eGFP). The expression level of eGFP was slightly higher when using two promoters (Psin2) than using original promoters. The Psin2 promoter was further engineered by modifying the repressor binding site and -35 and -10 regions. Shine-Dalgarno (SD) sequence of the sinI gene was modified to the consensus sequence. Finally, combining the engineered Psin2 promoter with the modified SD sequence increased the expression level of eGFP by about 13.4-fold over the original promoter. Our results suggest that the optimized sinIR promoter could be used as a novel tool for recombinant protein expression in B. subtilis. © The Korean Society for Applied Biological Chemistry 2023.
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