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通过可变剪接实现脂肪醛脱氢酶在内质网和过氧化物酶体中的双亚细胞定位以及在抵御氧化应激方面的重要作用。

Dual subcellular localization in the endoplasmic reticulum and peroxisomes and a vital role in protecting against oxidative stress of fatty aldehyde dehydrogenase are achieved by alternative splicing.

作者信息

Ashibe Bunichiro, Hirai Toshitake, Higashi Kyoichiro, Sekimizu Kazuhisa, Motojima Kiyoto

机构信息

Department of Biochemistry, Meiji Pharmaceutical University, Noshio 2-522-1, Kiyose, Tokyo 204-8588, Japan.

出版信息

J Biol Chem. 2007 Jul 13;282(28):20763-73. doi: 10.1074/jbc.M611853200. Epub 2007 May 16.

DOI:10.1074/jbc.M611853200
PMID:17510064
Abstract

Fatty aldehyde dehydrogenase (FALDH, ALDH3A2) is thought to be involved in the degradation of phytanic acid, a saturated branched chain fatty acid derived from chlorophyll. However, the identity, subcellular distribution, and physiological roles of FALDH are unclear because several variants produced by alternative splicing are present in varying amounts at different subcellular locations. Subcellular fractionation experiments do not provide a clear-cut conclusion because of the incomplete separation of organelles. We established human cell lines heterologously expressing mouse FALDH from each cDNA without tagging under the control of an inducible promoter and detected the variant FALDH proteins using a mouse FALDH-specific antibody. One variant, FALDH-V, was exclusively detected in peroxisomal membranes. Human FALDH-V with an amino-terminal Myc sequence also localized to peroxisomes. The most dominant form, FALDH-N, and other variants examined, however, were distributed in the endoplasmic reticulum. A gas chromatography-mass spectrometry-based analysis of metabolites in FALDH-expressing cells incubated with phytol or phytanic acid showed that FALDH-V, not FALDH-N, is the key aldehyde dehydrogenase in the degradation pathway and that it protects peroxisomes from oxidative stress. In contrast, both FALDHs had a protective effect against oxidative stress induced by a model aldehyde for lipid peroxidation, dodecanal. These results suggest that FALDH variants are produced by alternative splicing and share an important role in protecting against oxidative stress in an organelle-specific manner.

摘要

脂肪醛脱氢酶(FALDH,ALDH3A2)被认为参与植烷酸的降解,植烷酸是一种源自叶绿素的饱和支链脂肪酸。然而,由于可变剪接产生的几种变体在不同亚细胞位置的含量不同,FALDH的身份、亚细胞分布和生理作用尚不清楚。由于细胞器的分离不完全,亚细胞分级实验无法得出明确结论。我们建立了在诱导型启动子控制下从每个cDNA异源表达小鼠FALDH且不进行标记的人细胞系,并使用小鼠FALDH特异性抗体检测变体FALDH蛋白。一种变体FALDH-V仅在过氧化物酶体膜中被检测到。带有氨基末端Myc序列的人FALDH-V也定位于过氧化物酶体。然而,最主要的形式FALDH-N和其他检测的变体分布在内质网中。对用叶绿醇或植烷酸孵育的FALDH表达细胞中的代谢物进行基于气相色谱-质谱的分析表明,FALDH-V而非FALDH-N是降解途径中的关键醛脱氢酶,并且它能保护过氧化物酶体免受氧化应激。相比之下,两种FALDH对脂质过氧化模型醛十二醛诱导的氧化应激都有保护作用。这些结果表明,FALDH变体是由可变剪接产生的,并且以细胞器特异性方式在抵抗氧化应激中发挥重要作用。

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