关键词: HAL1基因 融合蛋白 表达 根瘤菌

Abstract:

Recombined plasmid pEGX-HAL1 was constructed using prokaryotic expression vector pGEX-4T-1, and transformed to Rhizobia by tri-parental mating to express fusion protein GST-HAL1. The results revealed that the salt resistance of engineered Rhizobia induced by IPTG was obviously improved, compared with blank and engineered Rhizobia without inducemeat. Under different temperatures, different inducing times and different IPTG inducement concentration, the expressing quantities of fusion protein were investigated to optimize the inducing parameters. The expressing quantities of fusion protein GST-HAL1 obviously increased under 28℃. Moreover, GST fusion protein can be induced effectively in engineered Rhizobia, and the product is up to 3.02 mg·L^-1liquuid medium, which is 39.34% of total soluble protein, under the inducing conditions of 3 h and 1.0 mmol·L^-1 IPTG concentration. The study may contribuute to bio-fertilizer production by utilizing gene engineering technology in the future.

Key words: HAL1 gene, fusion protein, expression, Rhizobia