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Isolation and immunofluorescent localization of actin derived from rat skeletal muscle
Authors:H. M. Abandowitz  P. K. Basrur
Affiliation:(1) Department of Biomedical Sciences, University of Guelph, Guelph, Ontario, Canada
Abstract:Summary Rat skeletal muscle actin was extracted, purified and its homogeneity established according to the criteria of ultracentrifugation and electrophoresis. Immunofluorescence procedure using antisera prepared in rabbits against the purified rat skeletal muscle actin revealed localized staining reaction in the I band region of the skeletal muscle. Similar studies on rat embryo muscle cultures showed a diffuse cytoplasmic fluorescence in fibroblastlike cells and an intense fluorescence in the multi-nucleated myoblasts of the younger cultures. In the older cultures strong fluorescence was detectable in scattered parallel rows and in the presumptive I bands of mononucleated myoblasts an in the thread-like mitochondria of fibroblasts. The distribution of fluorescence in these cells is considered indicative of the association of actin with the contracile protein in general and with mitochondria which in cultured myoblasts assume enormous lengths and appear to be extremely motile.
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