Optimization of cloning and expression of beta-glucanase gene from Bacillus amyloliquefaciens / 生物工程学报
Chinese Journal of Biotechnology
; (12): 542-548, 2009.
Article
in Zh
| WPRIM
| ID: wpr-286676
Responsible library:
WPRO
ABSTRACT
To compare of performance of beta-1,3-1,4-glucanase gene (bgl) in different expression systems, the beta-1,3-1,4-glucanase gene (GenBank Accession No. EU623974) was amplified from Bacillus amyloliquefaciens BS5582 by PCR and was cloned into three vectors pEGX-4T-1, pET20b(+) and pET28a(+) to construct pEGX-4T-1-bgl, pET20b(+)-bgl and pET28a(+)-bgl recombinant plasmids. The pEGX-4T-1-bgl was transformed into three different Escherichia coli host strains. The pET20b (+)-bgl and pET28a (+)-bgl were transformed into E. coli BL21 (DE3) respectively. Recombinant beta-glucanase was expressed by IPTG inducement in these recombinants. E. coli BL21 (DE3)-pET28a (+)-bgl had the highest enzyme activity. In Luria-Bertani medium, the total enzyme activity was (322.0 +/- 8.8) U/mL, which was 40.1% of original strain in optimal shaking flask condition. This recombinant's performance was studied in Terrific Broth medium under inducement of IPTG and lactose at the same time., and the highest total enzyme activity could reach (1883.3 +/- 45.8) U/mL (818.8% of the original), which indicate that the recombinant strain has a good value in industry application.
Full text:
1
Database:
WPRIM
Main subject:
Bacillus
/
Recombinant Proteins
/
Molecular Sequence Data
/
Cloning, Molecular
/
Endo-1,3(4)-beta-Glucanase
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Escherichia coli
/
Genetic Vectors
/
Genetics
/
Metabolism
Language:
Zh
Journal:
Chinese Journal of Biotechnology
Year:
2009
Document type:
Article