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糖基甘油二酯、甾醇糖苷和酰化甾醇糖苷的生物合成与结构

Biosynthesis and structure of glycosyl diglycerides, steryl glucosides, and acylated steryl glucosides.

作者信息

Elbein A D, Forsee W T

出版信息

Lipids. 1975 Jul;10(7):427-36. doi: 10.1007/BF02532449.

Abstract

A particulate enzyme fraction from Mycobacterim smegmatis catalyzed the transfer of -14C-glucose from the UDP--14C-glucose into neutral glycolipids. The two major radioactive components were purified by column chromatography on O-diethylamino ethyl cellulose (acetate) and thin layer chromatography on silica gel in several solvents. The first product yielded a water-soluble component upon saponification, which had a hexoseglycerol ratio of 1:1 with all of the hexose being identified as glucose. The second product yielded a water-soluble component upon saponification which contained hexose and glycerol in a 2:1 ratio and, in addition to glucose, contained lesser amounts of mannose and galactose. Palmitate and oleate were the predominant fatty acids and were present in equimolar amounts. The products thus have been identified as monoglycosyldiglyceride and diglycosyldiglyceride. The diglycosyldiglyceride could also be labeled with -14C-galactose when UDP--14C-galactose served as the donor, but the monoglycosyldiglyceride was only slightly labeled with -14C-galactose. Membrane fractions from mung bean seedlings catalyzed the transfer of -14C-glucose from UDP--14C-glucose into a neutral glycolipid which has been purified by thin layer chromatography and analyzed by combined gas liquid chromatography-mass spectrometry. It was determined to be a steryl glucoside with the two major sterol components being betasitosterol and stigmasterol linked to beta-D-glucose. Particulate fractions from developing cotton fibers also catalyzed the formation of steryl glucosides and, in addition, they catalyzed the esterification of steryl glucosides at the 6 position of glucose with fatty acids (primarily palmitate and oleate) from an andogenous acyl donor. Both the glucosyl transferase and the acyltransferase have been solubilized with Triton X-100 and partially purified by chromatography on Sephadex G-200. The acyltransferase activity was reconstituted by the addition of the steryl glucoside and a phospholipid acyl donor.

摘要

耻垢分枝杆菌的一种颗粒酶组分催化了 UDP - (^{14})C - 葡萄糖中(^{14})C - 葡萄糖向中性糖脂的转移。通过在 O - 二乙氨基乙基纤维素(醋酸盐)上进行柱色谱以及在硅胶上于几种溶剂中进行薄层层析,对两种主要放射性组分进行了纯化。第一种产物皂化后产生一种水溶性组分,其己糖与甘油的比例为 1:1,所有己糖均被鉴定为葡萄糖。第二种产物皂化后产生一种水溶性组分,其中己糖与甘油的比例为 2:1,除葡萄糖外,还含有少量的甘露糖和半乳糖。棕榈酸酯和油酸酯是主要的脂肪酸,且它们以等摩尔量存在。因此,这些产物已被鉴定为单糖基二甘油酯和二糖基二甘油酯。当 UDP - (^{14})C - 半乳糖作为供体时,二糖基二甘油酯也能用(^{14})C - 半乳糖进行标记,但单糖基二甘油酯仅被(^{14})C - 半乳糖轻微标记。绿豆幼苗的膜组分催化了 UDP - (^{14})C - 葡萄糖中(^{14})C - 葡萄糖向一种中性糖脂的转移,该中性糖脂已通过薄层层析纯化并通过气相色谱 - 质谱联用进行了分析。它被确定为一种甾醇葡萄糖苷,两种主要的甾醇成分是与β - D - 葡萄糖相连的β - 谷甾醇和豆甾醇。发育中的棉纤维的颗粒组分也催化了甾醇葡萄糖苷的形成,此外,它们还催化了甾醇葡萄糖苷在葡萄糖的 6 位与来自内源性酰基供体的脂肪酸(主要是棕榈酸酯和油酸酯)发生酯化反应。葡糖基转移酶和酰基转移酶都已用 Triton X - 100 溶解,并通过在 Sephadex G - 200 上进行色谱法进行了部分纯化。通过添加甾醇葡萄糖苷和磷脂酰基供体,使酰基转移酶活性得以重建。

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