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A Simple Purification Method of Vibrio cholerae Non‐O1 Hemagglutinin/Protease by Immunoaffinity Column Chromatography Using a Monoclonal Antibody
Author(s) -
Naka Atsuko,
Honda Takeshi,
Miwatani Toshio
Publication year - 1992
Publication title -
microbiology and immunology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.664
H-Index - 70
eISSN - 1348-0421
pISSN - 0385-5600
DOI - 10.1111/j.1348-0421.1992.tb02040.x
Subject(s) - vibrio cholerae , monoclonal antibody , affinity chromatography , hemagglutinin (influenza) , biology , protease , chromatography , vibrionaceae , microbiology and biotechnology , antibody , virology , biochemistry , bacteria , chemistry , enzyme , immunology , genetics , gene
A new simple purification method (I) for Vibrio cholerae non‐O1 hemagglutinin/protease (NAG‐HA/P) was developed. The method (I) requires only an immunoaffinity column chromatography using a monoclonal antibody against NAG‐HA/P. The method (I) is much simpler than previously reported purification method (II) (Honda, T. et al, Infection and Immunity 57: 2799–2803, 1989) which required four or more complicated chromatographic procedures. Method (I) also gave an improved recovery rate (about 27%) compared with (II), The molecular weight of NAG‐HA/P purified by method (I) was mainly 34 kilodaltons (kDa) with a little of 32 kDa, whereas that of NAG‐HA/P purified by (II) was usually 32 kDa. Immunological analysis by the Ouchterlony double gel diffusion test and Western blotting test using polyclonal antibody against 32 kDa protein revealed that the 34 and 32 kDa proteins are immunologically indistinguishable and thus it is supposed that 34 K protein is an isoform or a preform of the 32 K protein.