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Optimization and validation of a reversed-phase high performance liquid chromatography method for the measurement of bovine liver methylmalonyl-coenzyme a mutase activity

机译:反相高效液相色谱法测定牛肝甲基丙二酸辅酶A突变酶活性的优化与验证

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摘要

BackgroundMethylmalonyl-CoA mutase (MCM) is an adenosylcobalamin-dependent enzyme that catalyses the interconversion of (2R)-methylmalonyl-CoA to succinyl-CoA. In humans, a deficit in activity of MCM, due to an impairment of intracellular formation of adenosylcobalamin and methylcobalamin results in a wide spectrum of clinical manifestations ranging from moderate to fatal. Consequently, MCM is the subject of abundant literature. However, there is a lack of consensus on the reliable method to monitor its activity. This metabolic pathway is highly solicited in ruminants because it is essential for the utilization of propionate formed during ruminal fermentation. In lactating dairy cows, propionate is the major substrate for glucose formation. In present study, a reversed-phase high performance liquid chromatography (RP-HPLC) was optimized and validated to evaluate MCM activity in bovine liver. The major aim of the study was to describe the conditions to optimize reproducibility of the method and to determine stability of the enzyme and its product during storage and processing of samples.
机译:背景甲基丙二酰-CoA突变酶(MCM)是一种依赖腺苷钴胺素的酶,可催化(2R)-甲基丙二酰-CoA相互转化为琥珀酰-CoA。在人类中,由于腺苷钴胺素和甲基钴胺素的细胞内形成受损,MCM活性降低,导致多种临床表现,从中度到致命。因此,MCM是大量文献的主题。但是,对于监视其活动的可靠方法尚缺乏共识。反刍动物非常需要这种代谢途径,因为它对于利用瘤胃发酵过程中形成的丙酸至关重要。在泌乳的奶牛中,丙酸酯是葡萄糖形成的主要底物。在本研究中,反相高效液相色谱(RP-HPLC)已进行了优化和验证,以评估牛肝中MCM的活性。该研究的主要目的是描述条件,以优化该方法的可重复性,并确定样品及其在储存和加工过程中酶及其产物的稳定性。

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