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Serum LDL- and HDL-cholesterol determined by ultracentrifugation and HPLC

机译:通过超速离心和HPLC测定血清LDL和HDL胆固醇

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摘要

Simple and precise methods for LDL-cholesterol (LDL-C) and HDL-cholesterol (HDL-C) measurements are essential for assessment of cardiovascular disease (CVD) risks and for lipid and lipoprotein studies. We report here an ultracentrifugation (UC) and HPLC method that requires substantially less specimen volume and provides the necessary reliability and throughput required by large-volume, high-quality research and clinical studies. 2-Mercaptoethanol (ME) was used to dissociate serum lipoprotein [a] (Lp[a]) into apolipoprotein [a] and Lp[a] remnant (Lp[a−]) and eliminated the contamination of Lp[a] in HDL separated by UC. Serum aliquots were centrifuged at a density of 1.006 kg/l for the separation of HDL plus LDL, and in the presence of ME at a density of 1.063 kg/l for the separation of HDL. Cholesterol concentrations of the bottom fractions were analyzed by HPLC. LDL-C and HDL-C determined using this method were equivalent to those with β-quantification and the designated comparison method of the Centers for Disease Control. The total coefficient of variations for LDL-C and HDL-C were 0.65–1.12% and 0.96–2.07%, respectively. This method requires a small amount of specimen and is easy to operate. This method may be used in research or in clinical laboratories where precise and specific lipoprotein cholesterol analysis is needed.
机译:简单而精确的LDL-胆固醇(LDL-C)和HDL-胆固醇(HDL-C)测量方法对于评估心血管疾病(CVD)风险以及脂质和脂蛋白研究至关重要。我们在这里报告了一种超速离心(UC)和HPLC方法,该方法所需的样品量大大减少,并提供了大批量,高质量研究和临床研究所需的必要可靠性和通量。 2-巯基乙醇(ME)用于将血清脂蛋白[a](Lp [a])解离为载脂蛋白[a]和Lp [a]残留物(Lp [a-]),并消除了HDL中Lp [a]的污染由UC分隔。将血清等分试样以1.006 kg / l的密度离心以分离HDL和LDL,在有ME的情况下以1.063 kg / l的密度离心以分离HDL。通过HPLC分析底部馏分中的胆固醇浓度。用这种方法测定的LDL-C和HDL-C与用β-定量的那些和疾病控制中心指定的比较方法相同。 LDL-C和HDL-C的总变异系数分别为0.65-1.12%和0.96-2.07%。该方法需要少量的样品,并且易于操作。此方法可用于需要精确和特定脂蛋白胆固醇分析的研究或临床实验室。

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