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Attenuation of Slc27a5 gene expression followed by LC-MS measurement of bile acid reconjugation using metabolomics and a stable isotope tracer strategy
Authors:Castro-Perez Jose M  Roddy Thomas P  Shah Vinit  Wang Sheng-Ping  Ouyang Xuesong  Ogawa Anthony  McLaren David G  Tadin-Strapps Marija  Robinson Michael J  Bartz Steven R  Ason Brandon  Chen Ying  Previs Stephen F  Wong Kenny K  Vreeken Rob J  Johns Douglas G  Hubbard Brian K  Hankemeier Thomas  Mitnaul Lyndon
Institution:Merck Research Laboratories, Rahway, New Jersey, United States. jose_castro-perez@merck.com
Abstract:The purpose of this study was to evaluate the use of high resolution LC-MS together with metabolomics and D(4)-cholic acid (D(4)-CA) as a metabolic tracer to measure the metabolism and reconjugation of bile acids (BAs) in vitro and in vivo. Metabolic tracers are very important because they allow for the direct detection (substrate-to-product) of small and significant biological perturbations that may not be apparent when monitoring "static" endogenous levels of particular metabolites. Slc27a5, also known as fatty acid transport protein 5 (FATP5), is the hepatic BA-CoA ligase involved in reconjugating BAs during enterohepatic BA recycling. Using Slc27a5-cKD mice, silencing of ~90% gene expression was achieved followed by reduction in the reconjugation of D(4)-CA to D(4)-taurocholic acid (D(4)-TCA), as well as other conjugated BA metabolites in plasma (p = 0.0031). The method described allowed a rapid measure of many D(4) and endogenous BA. Analysis of bile resulted in the detection of 39 BA metabolites from a 13 min analytical run. Finally, the utilization of a novel high resolution mass spectrometry method in combination with metabolomics and a stable isotope metabolic tracer allowed for the detection of targeted and untargeted BAs following silencing of the Slc27a5 gene in primary hepatocytes and in mice.
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