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重塑途径和从头合成途径之间的串扰通过泛素化维持磷脂平衡。

Cross-talk between remodeling and de novo pathways maintains phospholipid balance through ubiquitination.

机构信息

Department of Biochemistry, Roy J. and Lucille A. Carver College of Medicine, University of Iowa, Iowa City, Iowa 52242, USA.

出版信息

J Biol Chem. 2010 Feb 26;285(9):6246-58. doi: 10.1074/jbc.M109.017350. Epub 2009 Dec 15.

Abstract

Phosphatidylcholine (PtdCho), the major phospholipid of animal membranes, is generated by its remodeling and de novo synthesis. Overexpression of the remodeling enzyme, LPCAT1 (acyl-CoA:lysophosphatidylcholine acyltransferase) in epithelia decreased de novo PtdCho synthesis without significantly altering cellular PtdCho mass. Overexpression of LPCAT1 increased degradation of CPT1 (cholinephosphotransferase), a resident Golgi enzyme that catalyzes the terminal step for de novo PtdCho synthesis. CPT1 degradation involved its multiubiquitination and processing via the lysosomal pathway. CPT1 mutants harboring arginine substitutions at multiple carboxyl-terminal lysines exhibited proteolytic resistance to effects of LPCAT1 overexpression in cells and restored de novo PtdCho synthesis. Thus, cross-talk between phospholipid remodeling and de novo pathways involves ubiquitin-lysosomal processing of a key molecular target that mechanistically provides homeostatic control of cellular PtdCho content.

摘要

磷脂酰胆碱(PtdCho)是动物膜的主要磷脂,由其重塑和从头合成产生。上皮细胞中重塑酶 LPCAT1(酰基辅酶 A:溶血磷脂酰胆碱酰基转移酶)的过表达降低了从头合成 PtdCho 的合成,而不会显著改变细胞内 PtdCho 的质量。LPCAT1 的过表达增加了 CPT1(胆碱磷酸转移酶)的降解,CPT1 是一种驻留的高尔基体酶,催化从头合成 PtdCho 的终末步骤。CPT1 的降解涉及通过溶酶体途径进行的多泛素化和加工。在细胞中,携带多个羧基末端赖氨酸的精氨酸取代突变的 CPT1 对 LPCAT1 过表达的影响具有抗蛋白水解作用,并恢复了从头合成 PtdCho。因此,磷脂重塑和从头合成途径之间的串扰涉及关键分子靶标的泛素-溶酶体加工,该途径从机制上提供了细胞 PtdCho 含量的体内平衡控制。

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