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A simple method for in vitro studies with rodent urinary blandders
Authors:C. D. Jackson  Glenn Newport
Affiliation:(1) Department of Health, Education and Welfare, Food and Drug Administration, National Center for Toxicological Research, 72079 Jefferson, Arkansas
Abstract:Summary A method was developed for the in vitro study of rodent urinary bladders. The method consists of everting and distending the urinary bladder in a manner to allow exposure of the luminal surface of the urothelium during in vitro incubation while maintaining the integrity of the structure and morphology of the bladder. A technique for selectively removing the urothelium with SDS buffer for biochemical analysis was described. Incorporation of [3H]leucine into urothelial protein was linear over a 4 h period in the presence of tissue culture medium, but no significant incorporation occurred when urine was used as incubation medium. Autoradiography indicated the [3H]leucine incorporation was almost exclusively in the urothelial cells with essentially no incorporation by cells below the tunica propria.
Keywords:mouse  urinary bladder  in vitro  autoradiography  leucine incorporation
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