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磷酸二羟丙酮酰基转移酶和烷基磷酸二羟丙酮合酶在大鼠肝脏过氧化物酶体中的特异性定位。

Exclusive localization in peroxisomes of dihydroxyacetone phosphate acyltransferase and alkyl-dihydroxyacetone phosphate synthase in rat liver.

作者信息

Singh H, Beckman K, Poulos A

机构信息

Department of Chemical Pathology, Adelaide Children's Hospital, Australia.

出版信息

J Lipid Res. 1993 Mar;34(3):467-77.

PMID:8468530
Abstract

Dihydroxyacetone phosphate acyl transferase (DHAP-AT), alkyl dihydroxyacetone phosphate synthase (alkyl-DHAP-synthase), and glycerol-3-phosphate acyltransferase (GPAT) activities were investigated under optimal assay conditions using highly purified organelle preparations. The data presented clearly indicate that GPAT activity was mainly localized in mitochondria and microsomes, whereas DHAP-AT and alkyl-DHAP-synthase activities were exclusively localized in peroxisomes. A small fraction of the total DHAP-AT and alkyl-DHAP-synthase activities observed in purified mitochondrial preparations was due to the presence of intact peroxisomes. DHAP-AT and alkyl-DHAP-synthase activities were very low in purified microsomes (< 1% compared to peroxisomes) and these activities are thought to be due to sedimentation of peroxisomal fragments (generated during homogenization of liver and processing of liver homogenate) with microsomes. The results indicate that the dihydroxyacetone phosphate pathway does not contribute to the synthesis of glycerolipids other than ether lipids in rat liver. The ether bond formation occurs exclusively in peroxisomes, and all the biosynthetic reactions for plasmalogen synthesis may also be operating within peroxisomes in rat liver.

摘要

在最佳测定条件下,使用高度纯化的细胞器制剂研究了磷酸二羟丙酮酰基转移酶(DHAP-AT)、烷基磷酸二羟丙酮合酶(烷基-DHAP-合酶)和甘油-3-磷酸酰基转移酶(GPAT)的活性。所呈现的数据清楚地表明,GPAT活性主要定位于线粒体和微粒体中,而DHAP-AT和烷基-DHAP-合酶活性仅定位于过氧化物酶体中。在纯化的线粒体制剂中观察到的总DHAP-AT和烷基-DHAP-合酶活性的一小部分是由于完整过氧化物酶体的存在。纯化的微粒体中DHAP-AT和烷基-DHAP-合酶活性非常低(与过氧化物酶体相比<1%),这些活性被认为是由于过氧化物酶体片段(在肝脏匀浆和肝脏匀浆处理过程中产生)与微粒体一起沉淀所致。结果表明,磷酸二羟丙酮途径对大鼠肝脏中除醚脂以外的甘油脂质合成没有贡献。醚键的形成仅发生在过氧化物酶体中,并且大鼠肝脏中缩醛磷脂合成的所有生物合成反应也可能在过氧化物酶体中进行。

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