Ribonuclease U2: cloning, production in Pichia pastoris and affinity chromatography purification of the active recombinant protein |
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| Authors: | Martínez-Ruiz A García-Ortega L Kao R Oñaderra M Mancheño J M Davies J Martínez del Pozo A Gavilanes J G |
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| Institution: | Department of Applied Biology, Faculty of Textile Science and Technology, Shinshu University, Tokida, Ueda-shi, Nagano, Japan. |
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| Abstract: | A recombinant lipase, CWB-LipB, localized on the Bacillus subtilis cell surface and retaining lipase activity was unstable and not accumulated in a high yield. To improve the accumulation, we examined cell wall binding protease (wprA)- and/or sigma D (sigD)-deficient mutants, and also a NprE and AprA protease-deficient mutant as host strains. The nprE aprA mutation did not lead to a significant increase in the CWB-LipB accumulation. The wprA mutant accumulated a greater amount than the wild-type only in the stationary phase, but the sigD mutant accumulated a greater amount in both the exponential and stationary phases. The double mutant exhibited great accumulation of CWB-LipB, the amount being 36% of the total proteins extracted from the cell surface. |
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| Keywords: | Bacillus subtilis Lipase Autolysin Surface engineering |
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