Site-specific mutagenesis of the catalytic subunit of cholera toxin: substituting lysine for arginine 7 causes loss of activity

Author:

Burnette W N1,Mar V L1,Platler B W1,Schlotterbeck J D1,McGinley M D1,Stoney K S1,Rohde M F1,Kaslow H R1

Affiliation:

1. Amgen Inc., Thousand Oaks, California 91320.

Abstract

Cholera and pertussis toxins each contain a subunit with ADP-ribosyltransferase activity, sharing a region of nearly identical amino acid sequence near the NH2 terminus. Previous investigations have shown that substitution of a lysine residue for Arg-9 in the catalytic A subunit of pertussis toxin substantially eliminates its enzyme activity. We now report that substitution of lysine for the position-equivalent Arg-7 of cholera toxin subunit A leads to a similar loss of catalytic activity. This result suggests a correlation of function with structure between the sequence-related cholera and pertussis toxin A subunits and may contribute to the design of a vaccine containing an enzymatically inert analog of cholera toxin.

Publisher

American Society for Microbiology

Subject

Infectious Diseases,Immunology,Microbiology,Parasitology

Reference33 articles.

1. Pertussis holotoxoid formed in vitro with a genetically deactivated S1 subunit;Bartley T. D.;Proc. Natl. Acad. Sci. USA,1989

2. The advent of recombinant pertussis vaccines;Burnette W. N.;Bio/Technology,1990

3. Burnette W. N. 1991. Perspectives in recombinant pertussis toxoid development p. 143-193. In H. R. Six and W. Koff(ed.) Vaccine research: a series of advances vol. 1. Marcel Dekker Inc. New York.

4. Pertussis toxin S1 mutant with reduced enzyme activity and a conserved protective epitope;Burnette W. N.;Science,1988

5. Direct expression of Bordetella pertussis toxin subunits to high levels in Escherichia coli;Burnette W. N.;Bio/Technology,1988

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