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人类 TMEM30a 促进抗肿瘤和生物活性胆碱磷脂进入哺乳动物细胞。

Human TMEM30a promotes uptake of antitumor and bioactive choline phospholipids into mammalian cells.

机构信息

Department of Cell Biology, Cleveland Clinic, Cleveland, OH 44195, USA.

出版信息

J Immunol. 2011 Mar 1;186(5):3215-25. doi: 10.4049/jimmunol.1002710. Epub 2011 Feb 2.

Abstract

Antitumor alkylphospholipids initiate apoptosis in transformed HL-60 and Jurkat cells while sparing their progenitors. 1-O-Alkyl-2-carboxymethyl-sn-glycero-3-phosphocholine (Edelfosine) like other short-chained phospholipids--inflammatory platelet-activating factor (PAF) and apoptotic oxidatively truncated phospholipids--are proposed to have intracellular sites of action, yet a conduit for these choline phospholipids into mammalian cells is undefined. Edelfosine is also accumulated by Saccharomyces cerevisiae in a process requiring the membrane protein Lem3p, and the human genome contains a Lem3p homolog TMEM30a. We show that import of choline phospholipids into S. cerevisiae ΔLem3 is partially reconstituted by human TMEM30a and by Lem3p-TMEM30a chimeras, showing the proteins are orthologous. TMEM30a-GFP chimeras expressed in mammalian cells localized in plasma membranes, as well as internal organelles, and ectopic TMEM30a expression promoted uptake of exogenous choline and ethanolamine phospholipids. Short hairpin RNA knockdown of TMEM30a reduced fluorescent choline phospholipid and [(3)H]PAF import. This knockdown also reduced mitochondrial depolarization from exogenous Edelfosine or the mitotoxic oxidatively truncated phospholipid azelaoyl phosphatidylcholine, and the knockdown reduced apoptosis in response to these two phospholipids. These results show that extracellular choline phospholipids with short sn-2 residues can have intracellular roles and sites of metabolism because they are transport substrates for a TMEM30a phospholipid import system. Variation in this mechanism could limit sensitivity to short chain choline phospholipids such as Edelfosine, PAF, and proapoptotic phospholipids.

摘要

抗肿瘤烷基磷脂在转化的 HL-60 和 Jurkat 细胞中诱导细胞凋亡,而对其前体细胞则具有保护作用。1-O-烷基-2-羧甲基-sn-甘油-3-磷酸胆碱(埃德拉福林)与其他短链磷脂一样——炎症血小板激活因子(PAF)和凋亡氧化截断磷脂——被认为具有细胞内作用部位,但这些胆碱磷脂进入哺乳动物细胞的途径尚不清楚。埃德拉福林也被酿酒酵母在需要膜蛋白 Lem3p 的过程中积累,人类基因组包含一个 Lem3p 同源物 TMEM30a。我们表明,进入 S. cerevisiaeΔLem3 的胆碱磷脂的导入部分由人类 TMEM30a 和 Lem3p-TMEM30a 嵌合体重新构成,表明这些蛋白质是同源的。在哺乳动物细胞中表达的 TMEM30a-GFP 嵌合体定位于质膜以及内部细胞器,并且异位 TMEM30a 表达促进外源性胆碱和乙醇胺磷脂的摄取。TMEM30a 的短发夹 RNA 敲低减少了荧光胆碱磷脂和 [(3)H]PAF 的摄取。这种敲低还减少了来自外源性埃德拉福林或促凋亡氧化截断磷脂酰胆碱的线粒体去极化,并且敲低减少了对这两种磷脂的细胞凋亡反应。这些结果表明,具有短 sn-2 残基的细胞外胆碱磷脂可以具有细胞内作用和代谢部位,因为它们是 TMEM30a 磷脂导入系统的转运底物。这种机制的变异可能会限制对短链胆碱磷脂(如埃德拉福林、PAF 和促凋亡磷脂)的敏感性。

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