| Literature DB >> 16233016 |
J Ni1, S Tokuyama, A Sogabe, Y Kawamura, Y Tahara.
Abstract
An efficient expression system for producing catalase in Bacillus was developed. A catalase was purified from Bacillus sp. TE124 and the catalase gene was cloned by plaque hybridization with a probe constructed from the N-terminal amino acid sequence of the enzyme. The gene, containing an open reading frame of 1452 bp, was subcloned into pHY300PLK for self-cloning into the organism. As a result, the production of catalase increased 20-fold over that of the parent strain.Entities:
Year: 2001 PMID: 16233016 DOI: 10.1263/jbb.91.422
Source DB: PubMed Journal: J Biosci Bioeng ISSN: 1347-4421 Impact factor: 2.894