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缩醛磷脂的酸性水解,随后进行高效液相色谱分析。

Acidic hydrolysis of plasmalogens followed by high-performance liquid chromatography.

作者信息

Murphy E J, Stephens R, Jurkowitz-Alexander M, Horrocks L A

机构信息

Department of Medical Biochemistry, Ohio State University, Columbus 43210.

出版信息

Lipids. 1993 Jun;28(6):565-8. doi: 10.1007/BF02536090.

Abstract

A simple, quantitative method for determining the plasmalogen content of small samples is reported here. The method uses the different susceptibility to acid-catalyzed hydrolysis of the alkyl, alkenyl and acyl linkages to separate the plasmalogen subclass from the other two non-labile subclasses. Hydrolysis of plasmenylethanolamine and plasmenylcholine was complete after 4 and 1 min of acid treatment, respectively. The acid-catalyzed hydrolysis did not alter the phospholipid fatty acid composition, making this method useful for fatty acid compositional analysis of the plasmalogen subclass. High-performance liquid chromatography was used for separations, and phospholipids were quantitated by assay of lipid phosphorus or by direct quantitation of peak area. Using this method, small amounts (10 nmol) of ethanolamine glycerophospholipid and choline glycerophospholipid are subjected to acid-catalyzed hydrolysis and subsequent separation of the resulting lysocompounds obtained from plasmalogens from the more acid-stable alkylacyl and diacyl glycerophospholipid fractions. Our values for plasmalogens from commercial preparations of choline and ethanolamine glycerophospholipids agree with literature values. The usefulness of the method is demonstrated for small glycerophospholipid samples that are equivalent to samples from cultured neural cells.

摘要

本文报道了一种测定小样本中缩醛磷脂含量的简单定量方法。该方法利用烷基、烯基和酰基键对酸催化水解的不同敏感性,将缩醛磷脂亚类与其他两种稳定的亚类分离。分别在酸处理4分钟和1分钟后,缩醛磷脂酰乙醇胺和缩醛磷脂酰胆碱的水解完全。酸催化水解不会改变磷脂脂肪酸组成,使得该方法可用于缩醛磷脂亚类的脂肪酸组成分析。采用高效液相色谱进行分离,通过脂质磷测定或直接定量峰面积对磷脂进行定量。使用该方法,将少量(10 nmol)的乙醇胺甘油磷脂和胆碱甘油磷脂进行酸催化水解,随后将缩醛磷脂产生的溶血化合物与更耐酸的烷基酰基和二酰基甘油磷脂部分分离。我们从商业制备的胆碱和乙醇胺甘油磷脂中测得的缩醛磷脂值与文献值相符。该方法对相当于培养神经细胞样本的小甘油磷脂样本的实用性得到了证明。

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