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直接测量125I标记脂蛋白中载脂蛋白B的比活性。

Direct measurement of apoprotein B specific activity in 125I-labeled lipoproteins.

作者信息

Le N A, Melish J S, Roach B C, Ginsberg H N, Brown W V

出版信息

J Lipid Res. 1978 Jul;19(5):578-84.

PMID:209113
Abstract

A method for determining apoprotein B specific activity in radioiodinated lipoproteins is described and validated. It utilizes organic solvents and tetramethylurea in the isolation of apoprotein B from other radiolabeled contaminants, both lipid and protein, in exogenously labeled VLDL. The contaminants are also removed from those lipoprotein classes subsequently derived from VLDL, namely IDL and LDL. The procedure requires approximately 50 microgram of apoB per analysis, allowing specific activity determinations in triplicate on 3-ml plasma samples with a standard error of less than 6%. Finally, data from a study of apoprotein B turnover in VLDL, IDL, and LDL in a human subject is presented to demonstrate the potential of this method in further elucidating the kinetic interrelationships between these lipoprotein classes.

摘要

描述并验证了一种测定放射性碘化脂蛋白中载脂蛋白B比活性的方法。该方法利用有机溶剂和四甲基脲从外源性标记的极低密度脂蛋白(VLDL)中的其他放射性标记污染物(包括脂质和蛋白质)中分离载脂蛋白B。这些污染物也从随后由VLDL衍生的脂蛋白类别,即中间密度脂蛋白(IDL)和低密度脂蛋白(LDL)中去除。该程序每次分析需要约50微克的载脂蛋白B,允许对3毫升血浆样品进行一式三份的比活性测定,标准误差小于6%。最后,展示了一项关于人类受试者中VLDL、IDL和LDL中载脂蛋白B周转的研究数据,以证明该方法在进一步阐明这些脂蛋白类别之间的动力学相互关系方面的潜力。

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