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Glucocorticoid regulation of two serine hydrolases in rat splenic lymphocytes in vitro
Authors:Richard G MacDonald  John A Cidlowski
Institution:1. Department of Biochemistry, University of Vermont College of Medicine, Burlington, VT 05405 U.S.A.
Abstract:A quantitative assay employing binding of 3H]diisopropylfluorophosphate (3H]DFP) and SDS-polyacrylamide gel electrophoresis was used to measure serine hydrolases in cell-free extracts from rat splenic lymphocytes. After labeling with 3H]DFP at pH 7, six major serine hydrolases are detected on 10% gels, having molecular weights of 78, 55, 34, 30, 28 and 17 (· 10?3). When labeled at pH 4, only four activities are measured, with Mr or 79, 55, 33 and 17 (· 10?3). Incubation of splenic lymphocytes for 8 h in vitro with 1 μM dexamethasone followed by 3H]DFP labeling at pH 7 produces a 91% increase in the 17000 3H]DFP. Hormone treatment for 8 h with subsequent labeling at pH 4 results in a 15% increase in the largest (78000) species, as well as 73% increase in the 17000 enzyme, compared with lysates from cells incubated without steroid. These effects are not observed after only 4 h of glucocorticoid exposure. Dexamethasone treatment for 8 h does not produce a decrease in any of these serine hydrolases, nor is there an apparent induction of new enzymes (i.e., having a molecular weight different from the preexisting species). Studies examining the effect of protease inhibitors on the 3H]DFP capacity of these proteins, show that the 17000 enzyme is sensitive to the protease inhibitor, pepstatin A, as well as the sulfhydryl reagents dithiothreitol and N-ethylmaleimide. These result suggest that this dexamethasone-responsive enzyme is a protease which requires a free thiol group for optimal activity. These findings are discussed with regard to the mechanism of glucocorticoid action in lymphocytes.
Keywords:Diisopropylfluorophosphate binding  Glucocorticoid  Serine hydrolase  Dexamethasone  Protein degradation  (Rat spleen lymphocyte)  DFP  diisopropylfluorophosphate  SDS  sodium dodecyl sulfate
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