Recombinant Expression and Purification of the Botulinum Neurotoxin Type A Translocation Domain

Autor: Lacy, D.Borden, Stevens, Raymond C.
Zdroj: Protein Expression and Purification; November 1997, Vol. 11 Issue: 2 p195-200, 6p
Abstrakt: Botulinum neurotoxin type A in its fully activated form exists as a dichain protein consisting of a 50-kDa light chain and a 100-kDa heavy chain linked by a disulfide bond (B. R. DasGupta and H. Sugiyama,Biochem. Biophys. Res. Commun.48, 108–112, 1972). The protein can be further subdivided into three functional domains: a catalytic domain corresponding to the light chain, a translocation domain associated with the N-terminal half of the heavy chain, and a binding domain as the C-terminal half. To facilitate further structural and functional studies on the mechanism of toxin translocation, we report here the recombinantEscherichia coliexpression and purification of the isolated translocation domain with a yield of 1 mg pure protein per 1 g cell paste. Circular dichroism, enzyme-linked immunosorbent assays, and preliminary crystallization experiments verify proper protein folding. This reagent should serve as a key tool in elucidating the mechanism of translocation and in determining how the catalytic domain, a large 50-kDa metalloprotease, is delivered to the cytosol.
Databáze: Supplemental Index