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JBC, Vol. 251, Issue 19, 6135-6141, Oct, 1976
Y. Ikeda and M. Steiner
A rapid and highly specific method for the isolation of human platelet
tubulin by immunosorption was developed. Platelet tubulin isolated by
successive cycles of polymerization was used as antigen. Densitometric
quantification of the antigen subjected to sodium dodecyl
sulfate-polyacrylamide gel electrophoresis revealed 96% tubulin of
molecular weight 55,000 and 4% high molecular weight proteins (mr = 240,000
to 250,000) which co-purified with platelet micrtobule protein. Platelet
tubulin bound 0.57 mumol of colchicine/100 mg of protein. Monospecific
antibody of human platelet tubulin was prepared in rabbits. After
absorption with tubulin co-purifying high molecular weight proteins, and
serum proteins, the rabbit anti-tubulin serum gave a single precipitin line
on double immunodiffusion against platelet tubulin and the high speed
supernatant of a platelet sonicate (platelet extract). The antiserum
precipitated the colchicine-binding activity of platelet extracts. The
gamma-globulin fraction of the absorbed antiserum was linked to an agarose
matrix. Platelet extracts applied to such immunosorptive columns showed the
disappearance of a single protein which was eluted with 0.5 g/liter of
Triton X-100 and identified as platelet tubulin. Its colchicine-binding
activity was retained in full. Electron microscopic examination revealed
that the ability of platelet tubulin to polymerize and form tubules was not
impaired in the presence of 0.5 g/liter of Triton X-100. This simple
isolation procedure of platelet tubulin has great advantages in terms of
purity and yield and can readily be adapted for use with other cell
systems.
Isolation of platelet microtubule protein by an immunosorptive method
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J. Morgan, L. Rodkey, and B. Spooner Quantitation of cytoplasmic tubulin by radioimmunoassay Science, August 5, 1977; 197(4303): 578 - 580. [Abstract] [PDF] |
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