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金莲花酶催化 UDP-α-d-葡萄糖形成β,1→4 葡聚糖。

The Formation of beta, 1 --> 4 Glucan from UDP-alpha-d-Glucose Catalyzed by a Phaseolus aureus Enzyme.

机构信息

Department of Chemistry, Ohio University, Athens, Ohio 45701.

出版信息

Plant Physiol. 1972 Sep;50(3):371-4. doi: 10.1104/pp.50.3.371.

Abstract

Particulate enzyme preparations from Phaseolus aureus hypocotyls catalyze the formation of an alkali insoluble beta, 1 --> 4 linked [(14)C]-glucan using UDP-alpha-d [(14)C]-glucose as substrate. Particulate enzymes prepared from root tissue also catalyzed the production of beta, 1 --> 4 glucan. UDP-beta-d-[(14)C]-glucose would not serve as a substrate for these enzymes. The presence or absence of beta, 1 --> 4 glucan synthetase activity was independent of tissue source, substrate concentration, or homogenization method.The particulate enzyme also catalyzes the formation of a beta, 1 --> 3 linked glucan from UDP-d glucose which is usually soluble in hot alkali. The solubility of the beta, 1 --> 3[(14)C]-glucan decreased when the enzyme was obtained from hypocotyls germinated at a higher temperature. The water-soluble material resulting from the catalyzed reaction includes a large proportion of what appears to be [(14)C]-laminaribiose, and smaller proportions of [(14)C]-laminaritriose and [(14)C]-glucose. There is no detectable quantity of [(14)C]-cellobiose or [(14)C]-cellotriose in the water-soluble material.

摘要

菜豆下胚轴的颗粒酶制剂催化 UDP-α-D-[(14)C]-葡萄糖作为底物形成不溶于碱的β,1 --> 4 连接 [(14)C]-葡聚糖。从根组织制备的颗粒酶也催化β,1 --> 4 葡聚糖的产生。UDP-β-D-[(14)C]-葡萄糖不能作为这些酶的底物。β,1 --> 4 葡聚糖合酶活性的存在与否与组织来源、底物浓度或匀浆方法无关。颗粒酶还催化 UDP-d 葡萄糖形成β,1 --> 3 连接的葡聚糖,通常在热碱中可溶。当酶从在较高温度下发芽的下胚轴中获得时,β,1 --> 3[(14)C]-葡聚糖的溶解度降低。催化反应产生的水溶性物质包括很大一部分似乎是 [(14)C]-松二糖,以及较小比例的 [(14)C]-松三糖和 [(14)C]-葡萄糖。在水溶性物质中没有检测到 [(14)C]-纤维二糖或 [(14)C]-纤维三糖的数量。

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