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首页> 外文期刊>Journal of Lipid Research >Aminopropyl solid phase extraction and 2 D TLC of neutral glycosphingolipids and neutral lysoglycosphingolipids.
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Aminopropyl solid phase extraction and 2 D TLC of neutral glycosphingolipids and neutral lysoglycosphingolipids.

机译:中性糖鞘脂和中性糖鞘糖脂的氨丙基固相萃取和二维DLC。

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摘要

Methods for isolation of neutral lysoglycosphingolipids (n-lyso-GSLs) such as glucosylsphingosine and galactosylsphingosine normally involve mild alkaline or acid hydrolysis followed by multiple chromatography steps, yielding relatively low recoveries of n-lyso-GSLs and neutral glycosphingolipids (n-GSLs). We now describe a new technique for isolating these compounds using one chromatography step, resulting in quantitative recovery of n-GSLs and n-lyso-GSLs. Lipids are extracted using a modified Folch procedure in which recovery is optimized by reextracting the Folch upper phase with water-saturated butanol. The extract is applied to an aminopropyl solid phase column from which both n-GSLs and n-lyso-GSLs elute in the same fraction. Separation is achieved using a new two-dimensional thin-layer chromatography procedure. The usefulness of this technique for biological samples was tested by examining Glc[4,5-(3)H]ceramide and Glc[4,5-(3)H]sphingosine accumulation in metabolically-labeled neurons treated with an inhibitor of lysosomal glucocerebrosidase. Accurate quantification of both lipids was obtained with Glc[4,5-(3)H]ceramide and Glc[4,5-(3)H]sphingosine accumulating at levels of 20 nmol/mg DNA and 40 pmol/mg DNA, respectively. This simple and rapid technique can therefore be used for the analysis of lyso-GSLs and GSLs in the same tissue, which may permit the determination of their metabolic pathways in normal and in pathological tissues, such as those taken from Gaucher and Krabbe's disease patients.
机译:分离中性溶血糖鞘脂(n-lyso-GSLs)的方法,例如葡萄糖基鞘氨醇和半乳糖基鞘氨醇,通常需要轻度的碱或酸水解,然后进行多个色谱步骤,回收率相对较低的n-溶酶-GSL和中性糖鞘脂(n-GSLs)回收率较低。现在我们描述一种使用一个色谱步骤分离这些化合物的新技术,从而定量回收n-GSLs和n-lyso-GSLs。使用改良的Folch程序提取脂质,其中可通过用水饱和的丁醇反萃取Folch上层相来优化回收率。将提取物上样到氨基丙基固相柱上,从该柱中同时洗脱n-GSL和n-lyso-GSL。使用新的二维薄层色谱程序可实现分离。通过检查溶酶体葡糖脑苷脂酶抑制剂治疗的代谢标记神经元中的Glc [4,5-(3)H]神经酰胺和Glc [4,5-(3)H]鞘氨醇积累,测试了该技术对生物样品的有用性。 。使用Glc [4,5-(3)H]神经酰胺和Glc [4,5-(3)H]神经鞘氨醇分别积累了20 nmol / mg DNA和40 pmol / mg DNA的含量,可以准确定量两种脂质。 。因此,这种简单,快速的技术可用于分析同一组织中的溶酶-GSL和GSL,从而可以确定它们在正常组织和病理组织中的代谢途径,例如从Gaucher和Krabbe's病患者身上获取的代谢途径。

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