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Regulation by Phospholipids and Kinetic Studies of Plant Membrane-Bound UDP-Glucose Sterol β-d-Glucosyl Transferase

机译:磷脂调节和植物膜结合UDP-葡萄糖甾醇β-d-葡萄糖基转移酶的动力学研究

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摘要

Solubilization and partial purification of the microsomal UDP-glucose sterol glucosyl transferase activity from maize coleoptiles by chromatography on DEAE-cellulose resulted in a highly delipidated (>95%) and inactive enzymic preparation. Addition of sterols revealed part of the activity and subsequent addition of phospholipids further increased the activity. Negatively charged phospholipids were shown to be by far the best activators. The purification step also produced the elimination of two interfering microsomal enzymic activities: UDPase and steryl glucoside acyl transferase. The removal of these two enzymic activities was a prerequisite for kinetic studies including product-inhibition studies, since the substrates of these two latter enzymes are the products of UDPG-SGTase activity. The results of the kinetic studies strongly suggest an ordered bi-bi mechanism for the glucosylation of sterols. Finally the effect of different phospholipids on the kinetic parameters of the reaction was studied. Both phosphatidylcholine and phosphatidylglycerol significantly decrease Km-sterol (and not Km-UDPglucose) and increase the reaction Vmax. The decrease of Km-sterol is similar with both phospholipids whereas the increase of Vmax is much greater with phosphatidylglycerol than with phosphatidylcholine.
机译:通过在DEAE-纤维素上的色谱法从玉米胚芽鞘中溶解和部分纯化微粒体UDP-葡萄糖固醇葡糖基转移酶活性,导致高度脂质化(> 95%)和无活性的酶制剂。添加固醇显示出部分活性,随后添加磷脂进一步提高了活性。迄今为止,带负电荷的磷脂是最好的活化剂。纯化步骤还消除了两种干扰的微粒体酶活性:UDPase和甾基葡糖苷酰基转移酶。除去这两种酶活性是动力学研究(包括产物抑制研究)的前提条件,因为后两种酶的底物是UDPG-SGTase活性的产物。动力学研究的结果强烈暗示了固醇的糖基化的有序的双-bi机理。最后研究了不同磷脂对反应动力学参数的影响。磷脂酰胆碱和磷脂酰甘油都显着降低Km-固醇(而不是Km-UDP葡萄糖)并增加反应Vmax。两种磷脂中Km-固醇的减少都相似,而磷脂酰甘油的Vmax的增加比磷脂酰胆碱的大得多。

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