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基于替代物分析的 UPLC-MS/MS 法准确定量大鼠结肠息肉(Pirc)模型中的 PGE。

Accurate quantification of PGE in the polyposis in rat colon (Pirc) model by surrogate analyte-based UPLC-MS/MS.

机构信息

Department of Pharmacological and Pharmaceutical Sciences, University of Houston, 1441 Moursund St., Houston, TX, 77030, USA.

Center for Epigenetics & Disease Prevention, Texas A&M College of Medicine, 2121 W. Holcombe Blvd., Houston, TX, 77030, USA.

出版信息

J Pharm Biomed Anal. 2018 Jan 30;148:42-50. doi: 10.1016/j.jpba.2017.07.025. Epub 2017 Jul 25.

Abstract

An accurate and reliable UPLC-MS/MS method is reported for the quantification of endogenous Prostaglandin E2 (PGE) in rat colonic mucosa and polyps. This method adopted the "surrogate analyte plus authentic bio-matrix" approach, using two different stable isotopic labeled analogs - PGE-d9 as the surrogate analyte and PGE-d4 as the internal standard. A quantitative standard curve was constructed with the surrogate analyte in colonic mucosa homogenate, and the method was successfully validated with the authentic bio-matrix. Concentrations of endogenous PGE in both normal and inflammatory tissue homogenates were back-calculated based on the regression equation. Because of no endogenous interference on the surrogate analyte determination, the specificity was particularly good. By using authentic bio-matrix for validation, the matrix effect and exaction recovery are identically same for the quantitative standard curve and actual samples - this notably increased the assay accuracy. The method is easy, fast, robust and reliable for colon PGE determination. This "surrogate analyte" approach was applied to measure the Pirc (an Apc-mutant rat kindred that models human FAP) mucosa and polyps PGE, one of the strong biomarkers of colorectal cancer. A similar concept could be applied to endogenous biomarkers in other tissues.

摘要

本文报道了一种准确可靠的 UPLC-MS/MS 方法,用于定量检测大鼠结肠黏膜和息肉中的内源性前列腺素 E2(PGE)。该方法采用“替代分析物加真实生物基质”的方法,使用两种不同的稳定同位素标记类似物-PGE-d9 作为替代分析物和 PGE-d4 作为内标。在结肠黏膜匀浆中用替代分析物构建定量标准曲线,并使用真实生物基质对方法进行成功验证。根据回归方程,反推出正常和炎症组织匀浆中内源性 PGE 的浓度。由于替代分析物的测定不受内源性干扰,因此特异性特别好。通过使用真实生物基质进行验证,定量标准曲线和实际样品的基质效应和提取回收率完全相同-这显著提高了测定的准确性。该方法简单、快速、稳健且可靠,适用于结肠 PGE 的测定。这种“替代分析物”方法应用于测量 Pirc(一种模拟人类 FAP 的 APC 突变大鼠种系)黏膜和息肉中的 PGE,这是结直肠癌的一个强有力的生物标志物。类似的概念可以应用于其他组织中的内源性生物标志物。

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