4.3 Review

Functional expression of human cytochrome P450 enzymes in Escherichia coli

Journal

CURRENT DRUG METABOLISM
Volume 7, Issue 4, Pages 411-429

Publisher

BENTHAM SCIENCE PUBL LTD
DOI: 10.2174/138920006776873472

Keywords

cytochrome P450; NADPH-P450 oxidoreductase; heterologous expression; Escherichia coli; temperature effect; molecular chaperone

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Knowledge regarding cytochrome P450 (P450) is crucial to the fields of drug therapy and drug development, as well as in our understanding of the mechanisms underlying the metabolic activation of potentially toxic and carcinogenic compounds. Escherichia coli is the most extensively utilized host in the production of recombinant human 11450 enzymes. However, the recover), of substantial yields of functionally active P450 proteins remains problematic. Mammalian P450 protein was first expressed in 1991, via the modification of the N-terminal amino acid sequences in E. coli cells. Since that time, a variety of strategies have been established for the functional expression of recombinant P450s in E. coli, including N-terminat modification, the use of molecular chaperones. and Culturing at lower temperatures. In all cases, human P450 expressed in E. coli cells has been shown to efficiently catalyze the oxidation of representative substrates at efficient rates. These recombinant P450s are applicable to studies which estimate the kinetic parameters of drug oxidation, and have also been used to determine the metabolic pathways of drugs and carcinogens exploited by human P450s. Despite the potential of P450s in various pharmaceutical and biotechnological fields. however. a host of substantial challenges must be overcome before these enzymes can be routinely utilized. Intrinsically, these enzymes are not very active. and exhibit poor stability. in this review, we have described current developments in the heterolopous expression of human P450 enzymes.

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