Ivor Smith scite author profile

Proteins secreted by strains of Mycobacterium tuberculosis during short-term, zinc-sufficient batch culture were identified in order to define antigens likely to be relevant to the pathogenesis of human disease. [35S]Methionine-labelled proteins in supernatants of 4-7 d cultures were separated by PAGE under both denaturing and non-denaturing conditions, and the position of labelled material was determined. Secreted protein patterns of M. tuberculosis were quite similar to those of Bacillus Calmette-Guérin (BCG) but differed by the absence of the 46 kDa dimeric protein specific to BCG and by the presence in large amounts of a 23 kDa protein which, when denatured, gave 13 kDa subunits. This 13 kDa subunit protein constituted up to 20% of secreted proteins in classical strains of M. tuberculosis of phage type B but was not detected in phage type I strains from South India. This may be relevant to the different pathogenicity of these strains. Western blot analysis showed that antigens defined in supernatants of short-term (3 d) cultures of M. tuberculosis constituted a small subset of those seen in supernatants of organisms cultured for longer periods. One of the secreted proteins has the interesting property of binding to fibronectin. The available monoclonal antibodies and antisera have been used to identify lines on immunoblots corresponding to the secreted/released antigens of M. tuberculosis. The present findings suggest that there are major secreted antigens to which antibodies do not yet appear to have been produced experimentally.

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Acrylamide Gel Disc Electrophoresis

Smith¹

1968

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A monoclonal antibody to T-2 toxin

Goodbrand¹,

Stimson²,

Smith³

1987

Lett Appl Microbiol

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A specific, high affinity monoclonal antibody to T‐2 toxin of Fusarium has been produced. The monoclonal antibody was conjugated to horse‐radish peroxidase and employed to develop a direct competitive enzyme‐linked immunosorbent assay (ELISA) for the toxin. The sensitivity of the ELISA was 10 ng/ml with a working range up to 500 ng/ml. The antibody cross‐reacted with HT‐2 toxin (25%) but did not bind to any other trichothecene tested.

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Starch Gel Electrophoresis

Smith¹

1968

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Seeing gel wells well

Smith

Cromie

Stainsby

1988

Analytical Biochemistry

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Ivor Smith

The Secreted Antigens of Mycobacterium tuberculosis and Their Relationship to Those Recognized by the Available Antibodies

Acrylamide Gel Disc Electrophoresis

A monoclonal antibody to T-2 toxin

Starch Gel Electrophoresis

Seeing gel wells well

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