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甘露糖基磷酸多萜醇的水溶性类似物的跨膜运动由一种内质网蛋白介导。

Transmembrane movement of a water-soluble analogue of mannosylphosphoryldolichol is mediated by an endoplasmic reticulum protein.

作者信息

Rush J S, Waechter C J

机构信息

Department of Biochemistry, University of Kentucky College of Medicine, Lexington 40536, USA.

出版信息

J Cell Biol. 1995 Aug;130(3):529-36. doi: 10.1083/jcb.130.3.529.

Abstract

Based on topological studies mannosylphosphoryldolichol (Man-P-Dol) is synthesized on the cytoplasmic face of the RER, but functions as a mannosyl donor in Glc3Man9GlcNAc2-P-P-dolichol biosynthesis after the mannosyl-phosphoryl headgroup diffuses transversely to the luminal compartment. The transport of mannosylphosphorylcitronellol (Man-P-Cit), a water-soluble analogue of Man-P-Dol, by microsomal vesicles from mouse liver, has been investigated as a potential experimental approach to determine if a membrane protein(s) mediates the transbilayer movement of Man-P-Dol. For these studies beta-[3H]Man-P-Cit was synthesized enzymatically with a partially purified preparation of Man-P-undecaprenol synthase from Micrococcus luteus. The uptake of the radiolabeled water-soluble analogue was found to be (a) time dependent; (b) stereoselective; (c) dependent on an intact permeability barrier; (d) saturable; (e) protease-sensitive; and (f) highest in ER-enriched vesicles relative to Golgi complex-enriched vesicles and intact mitochondria. Consistent with the involvement of a membrane protein, the analogue did not enter synthetic phosphatidylcholine-liposomes. [3H]Man-P-Cit also was not transported by human erythrocytes. These results indicate that the transport of Man-P-Cit by sealed microsomal vesicles from mouse liver is mediated by a membrane protein transport system. It is possible that the same membrane protein(s) participates in the transbilayer movement of Man-P-Dol in the ER.

摘要

基于拓扑学研究,甘露糖基磷酸多萜醇(Man-P-Dol)在糙面内质网(RER)的胞质面合成,但在甘露糖基磷酸头部基团横向扩散到内质网腔后,它在Glc3Man9GlcNAc2-P-P-多萜醇生物合成中作为甘露糖基供体发挥作用。甘露糖基磷酸香茅醇(Man-P-Cit)是Man-P-Dol的水溶性类似物,对来自小鼠肝脏的微粒体囊泡运输Man-P-Cit进行了研究,以此作为一种潜在的实验方法来确定是否有膜蛋白介导Man-P-Dol的跨膜运动。在这些研究中,用来自藤黄微球菌的部分纯化的Man-P-十一异戊烯醇合酶制剂酶促合成了β-[3H]Man-P-Cit。发现放射性标记的水溶性类似物的摄取具有以下特点:(a)时间依赖性;(b)立体选择性;(c)依赖于完整的通透性屏障;(d)可饱和;(e)对蛋白酶敏感;(f)相对于富含高尔基体复合体的囊泡和完整线粒体,在富含内质网的囊泡中摄取量最高。与膜蛋白的参与一致,该类似物不进入合成的磷脂酰胆碱脂质体。[3H]Man-P-Cit也不能被人红细胞运输。这些结果表明,来自小鼠肝脏的封闭微粒体囊泡对Man-P-Cit的运输是由膜蛋白运输系统介导的。有可能相同的膜蛋白参与内质网中Man-P-Dol的跨膜运动。

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