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首页> 外文期刊>Clinical Biochemistry >Determination of free and total carnitine in plasma by an enzymatic reaction and spectrophotometric quantitation spectrophotometric determination of carnitine.
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Determination of free and total carnitine in plasma by an enzymatic reaction and spectrophotometric quantitation spectrophotometric determination of carnitine.

机译:酶促反应和分光光度定量光度法测定肉碱中血浆中游离和总肉碱的含量。

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OBJECTIVES: Carnitine initiates the beta-oxidation of fatty acids and its deficiency is a problem in several metabolic diseases. This work describes a validated quick and simple enzymatic assay for the determination of free and total carnitine in plasma. METHODS: Carnitine reacts with acetyl-CoA catalized by carnitine acetyltransferase. The coenzyme A liberated combines with 5,5'-dithiobis-(2-nitrobenzoic acid) and forms thiophenolate ion, measured spectrophotometrically at 412 nm. The method requires precipitation of proteins and the alkaline hydrolysis of acylcarnitines for total carnitine. RESULTS: The detection limit is 1.7 micromol/L in plasma and inter- and intra-day imprecision is less than 5%. The recovery of spiked plasma samples is 97%. The method was tested with an inter-laboratory assay, yielding excellent correlation (r(2)=0.994), and it was applied to the determination of normal values of carnitine in plasma. CONCLUSIONS: A reliable spectrophotometric method has been validated with very good precision, with simple instrumental and easy sample preparation.
机译:目的:肉碱会引发脂肪酸的β-氧化作用,其缺乏是几种代谢疾病中的一个问题。这项工作描述了一种经过验证的快速简便的酶法测定血浆中游离和总肉碱的方法。方法:肉碱与肉碱乙酰基转移酶催化的乙酰辅酶A反应。所释放的辅酶A与5,5'-二硫代双-(2-硝基苯甲酸)结合并形成硫酚酸根离子,在412 nm处用分光光度法测量。该方法需要蛋白质沉淀和酰基肉碱的碱水解才能制成总肉碱。结果:血浆中的检出限为1.7 micromol / L,日间和日内不精确度小于5%。加标血浆样品的回收率为97%。该方法通过实验室间试验进行测试,产生了极好的相关性(r(2)= 0.994),并用于测定血浆中肉碱的正常值。结论:已经验证了一种可靠的分光光度法,具有很高的精密度,且仪器简单且样品制备简单。

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