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. 1989 Feb 28;159(1):87-94.
doi: 10.1016/0006-291x(89)92408-x.

Chemical synthesis and expression of the HIV-1 protease gene in E. coli

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Chemical synthesis and expression of the HIV-1 protease gene in E. coli

J M Louis et al. Biochem Biophys Res Commun. .

Abstract

The 297bp HIV-1 protease gene was constructed from five discrete synthetic fragments and expressed in E. coli. A soluble protein product of 11.5 Kd was detected by immunoblotting using protease specific antisera. A quantitative assay system, utilizing a synthetic nonapeptide spanning the cleavage site between p17-p24 in the gag polyprotein, was used to measure the specific protease activity in crude extracts. The protease hydrolyzed tyrosyl-proline bonds with an approximate specific activity of 43 pmoles/min/micrograms of total protein. The chemical synthesis of the protease gene and it's expression provides a feasible method for rapid mutant analysis, important for structure-function studies and rational design of potential inhibitors.

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