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LC-MS/MS 定量检测磺基转移酶比传统免疫法更能准确反映人肝 SULT 活性:精准医学的启示

LC-MS/MS quantification of sulfotransferases is better than conventional immunogenic methods in determining human liver SULT activities: implication in precision medicine.

机构信息

Department of Pharmaceutics, School of Pharmaceutical Sciences, Southern Medical University, Guangzhou, Guangdong, 510515, China.

International Institute for Translational Chinese Medicine, Guangzhou University of Chinese Medicine, Guangzhou, Guangdong, 510006, China.

出版信息

Sci Rep. 2017 Jun 20;7(1):3858. doi: 10.1038/s41598-017-04202-w.

Abstract

This study aims to determine whether enzyme activities are correlated with protein amounts and mRNA expression levels of five major human sulfotransferase (SULT) enzymes in 10 matched pericarcinomatous and hepatocellular carcinoma liver samples. The MRM UHPLC-MS/MS method, Western blot and RT-PCR were used along with SULT activity measurement using probe substrates. The LC-MS/MS method was specific for all five tested SULTs, whereas Western blot was specific for only two isoforms. The activities of SULT1A1, SULT1B1, SULT1E1 and SULT2A1 in 9 of 10 samples showed a significant decrease in tumor tissues relative to matched pericarcinomatous tissues, whereas the activities of SULT1A3 in 7 of 10 samples increased. The turnover numbers of SULTs did not change, except for SULT1A1. A generally high degree of correlations was observed between SULT activities and protein amounts (r ≥ 0.59 except one), whereas a low degree of correlations was observed between SULT activities and mRNA expression levels (r ≤ 0.48 except one). HCC reduced the SULT activities via impaired protein amounts. LC-MS/MS quantification of SULTs is highly reliable measurement of SULT activities, and may be adopted for implementing precision medicine with respect to drugs mainly metabolized by SULTs in healthy and HCC patients.

摘要

本研究旨在确定在 10 对配对的癌旁组织和肝癌组织样本中,五种主要人类磺基转移酶(SULT)的酶活性是否与蛋白质含量和 mRNA 表达水平相关。采用 MRM UHPLC-MS/MS 法、Western blot 和 RT-PCR 法,以及使用探针底物测量 SULT 活性。LC-MS/MS 方法对所有五种测试的 SULT 均具有特异性,而 Western blot 仅对两种同工酶具有特异性。在 10 个样本中的 9 个样本中,SULT1A1、SULT1B1、SULT1E1 和 SULT2A1 的活性在肿瘤组织中相对于配对的癌旁组织显著降低,而 SULT1A3 的活性在 7 个样本中增加。除 SULT1A1 外,SULT 的周转数没有变化。除一个外,SULT 活性与蛋白质含量之间观察到高度相关(r≥0.59),而 SULT 活性与 mRNA 表达水平之间的相关性较低(r≤0.48,除一个外)。HCC 通过减少蛋白质含量降低了 SULT 活性。LC-MS/MS 定量 SULT 是 SULT 活性的高度可靠测量方法,可用于在健康和 HCC 患者中实施主要由 SULT 代谢的药物的精准医学。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/754e/5478605/75cd6091ef73/41598_2017_4202_Fig1_HTML.jpg

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