| Literature DB >> 6092221 |
K Shigesada, N Tsurushita, Y Matsumoto, M Imai.
Abstract
A plasmid system has been constructed which allows high-level expression of the rho gene of Escherichia coli under the control of the pL promoter and the N-antitermination regulatory system of bacteriophage lambda. The pL-directed synthesis of Rho crucially depends on the lambda N gene product and is promoted most effectively when this product is supplied from the N gene cloned on a separate compatible plasmid with a moderate copy number. The requirement for N can be circumvented partly, but not completely, by deletion of the region preceding the rho structural gene. Attempts were also made to optimize the construction of rho-expression plasmids by adjusting the orientation and location of pL and rho inserts on the pBR322 vector. With optimal conditions, Rho protein is overexpressed 100-fold and can become as much as 10% of the total cellular protein. Using this plasmid system, Rho can be purified with a yield of more than 20 mg from 10 g of induced cells.Entities:
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Year: 1984 PMID: 6092221 DOI: 10.1016/0378-1119(84)90180-x
Source DB: PubMed Journal: Gene ISSN: 0378-1119 Impact factor: 3.688