In a batch cultivation of Pichia pastoris expressing Candida rugosa lipase 1 (CRL1), secretion of 200 ¿g lipase ml¿1 of culture was achieved in sorbitol-based medium. However, a large amount of recombinant protein was retained intracellularly throughout the fermentation, pointing to the transport step as a major bottleneck. Therefore a translational fusion with the green fluorescent protein (GFP) was constructed that was expressed and transported similarly to the native lipase and retained catalytic activity. This analytical tool enables a rapid monitoring of product localization and amount, based on GFP-associated fluorescence
Passolunghi, S., Brocca, S., Cannizzaro, L., Porro, D., Lotti, M. (2003). Monitoring the transport of recombinant Candida rugosa lipase by a green fluorescent protein-lipase fusion. BIOTECHNOLOGY LETTERS, 25(22), 1945-1948 [10.1023/B:BILE.0000003991.71854.09].
Monitoring the transport of recombinant Candida rugosa lipase by a green fluorescent protein-lipase fusion
Passolunghi, S;Brocca, S;Porro, D;Lotti, M
2003
Abstract
In a batch cultivation of Pichia pastoris expressing Candida rugosa lipase 1 (CRL1), secretion of 200 ¿g lipase ml¿1 of culture was achieved in sorbitol-based medium. However, a large amount of recombinant protein was retained intracellularly throughout the fermentation, pointing to the transport step as a major bottleneck. Therefore a translational fusion with the green fluorescent protein (GFP) was constructed that was expressed and transported similarly to the native lipase and retained catalytic activity. This analytical tool enables a rapid monitoring of product localization and amount, based on GFP-associated fluorescence
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