Department of Chemistry, National Cheng Kung University, Tainan, Taiwan.
J Proteomics. 2011 Nov 18;74(12):2734-44. doi: 10.1016/j.jprot.2011.01.015. Epub 2011 Feb 12.
Liver microsomes are subcellular fractions that contain many metabolizing enzymes for drugs and endogeneous compounds. Some of these enzymes are regulated by sex hormonal control and exhibit sex-dependent expression pattern and metabolizing speed. Studying these enzymes, however, are complicated by the presence of isoforms such as cytochrome P450 (CYP450), which families share more than 50% amino acid identities. In this study, we applied quantitative shot-gun proteomics approach coupled with stable-isotope dimethyl labeling, two-dimensional reversed-phase peptide separation and tandem mass spectrometry (MS) to explore the gender-dependent expression of rat liver microsomal proteins. A total of 391 proteins were identified and quantified by this approach, and 56% of quantified proteins were enzymes. Although shot-gun approach is rarely used for identifying protein isoforms, we identified 53 isoforms by at least one unique peptide including 21 isoforms of CYP450s. Moreover, by quantitative and statistics assessment, we were able to classify them into 28 male dominant enzymes including CYP2C12 CYP2C11, CYP2C13, CYP2B3, CYP2C11, CYP2C70 and CYP3A2 which are known to be male specific, 21 female dominant enzymes including CYP2A1, CYP2C7, CYP2C12, CYP2D26, alcohol dehydrogenase 1, carboxylesterase 3, glutathione S-transferase, liver carboxylesterase 4, UDP-glucuronosyltransferase 2B1, and glyceraldehyde-3-phosphate dehydrogenase which are known to be female specific; and 125 sex-independent enzymes. However, most of the sex specificities revealed from this study, such as the male specificity of CYP2D1, were novel and not yet reported. We then conducted a mass spectrometry-multiple reaction mode (MS-MRM) based enzyme activity method to determine the catalyzing rate of CYP2D1 in male and female liver microsomes using carteolol as its specific substrate. The reaction rate catalyzed by CYP2D1 in female rats was determined to differ significantly with the rate in male rats. Moreover, the ratio (female/male) of reaction rate (0.68) was found to correlate with their relative protein abundance (0.72). This study revealed novel sex dependences of many rat liver enzymes and also demonstrated a unique MS-based analytical platform that could identify novel iso-enzymes and further quantify their abundance and enzyme activity.
肝微粒体是含有许多药物和内源性化合物代谢酶的亚细胞部分。其中一些酶受性激素调控,表现出性别依赖性表达模式和代谢速度。然而,研究这些酶很复杂,因为存在同工酶,如细胞色素 P450(CYP450),其家族的氨基酸同一性超过 50%。在这项研究中,我们应用定量鸟枪法蛋白质组学方法结合稳定同位素二甲基标记、二维反相肽分离和串联质谱(MS)技术来探索大鼠肝微粒体蛋白的性别依赖性表达。通过这种方法共鉴定和定量了 391 种蛋白质,其中 56%的定量蛋白质为酶。尽管鸟枪法很少用于鉴定蛋白质同工酶,但我们通过至少一个独特肽鉴定了 53 个同工酶,包括 21 个 CYP450 同工酶。此外,通过定量和统计学评估,我们能够将它们分为 28 种雄性优势酶,包括 CYP2C12、CYP2C11、CYP2C13、CYP2B3、CYP2C11、CYP2C70 和 CYP3A2,这些酶已知是雄性特异性的;21 种雌性优势酶,包括 CYP2A1、CYP2C7、CYP2C12、CYP2D26、醇脱氢酶 1、羧酸酯酶 3、谷胱甘肽 S-转移酶、肝羧酸酯酶 4、UDP-葡糖醛酸基转移酶 2B1 和甘油醛-3-磷酸脱氢酶,这些酶已知是雌性特异性的;以及 125 种性别非依赖性酶。然而,这项研究揭示的大多数性别特异性,如 CYP2D1 的雄性特异性,都是新的,尚未报道。然后,我们使用卡替洛尔作为其特异性底物,通过基于质谱的多重反应模式(MS-MRM)酶活性方法来确定雄性和雌性肝微粒体中 CYP2D1 的催化速率。CYP2D1 在雌性大鼠中的催化速率与雄性大鼠中的催化速率有显著差异。此外,反应速率的比值(雌性/雄性)(0.68)与它们的相对蛋白丰度(0.72)相关。这项研究揭示了许多大鼠肝酶的新的性别依赖性,并证明了一种独特的基于 MS 的分析平台,可以识别新的同工酶,并进一步定量它们的丰度和酶活性。
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