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Mitochondrial Phosphatidylserine Decarboxylase from Higher Plants. Functional Complementation in Yeast Localization in Plants and Overexpression in Arabidopsis

机译:来自高等植物的线粒体磷脂酰丝氨酸脱羧酶。 酵母中的功能互补植物中的定位和 过度表达 拟南芥

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摘要

Plants are known to synthesize ethanolamine (Etn) moieties by decarboxylation of free serine (Ser), but there is also some evidence for phosphatidyl-Ser (Ptd-Ser) decarboxylation. Database searches identified diverse plant cDNAs and an Arabidopsis gene encoding 50-kD proteins homologous to yeast (Saccharomyces cerevisiae) and mammalian mitochondrial Ptd-Ser decarboxylases (PSDs). Like the latter, the plant proteins have putative mitochondrial targeting and inner membrane sorting sequences and contain near the C terminus a Glycine-Serine-Threonine motif corresponding to the site of proteolysis and catalytic pyruvoyl residue formation. A truncated tomato (Lycopersicon esculentum) cDNA lacking the targeting sequence and a chimeric construct in which the targeting and sorting sequences were replaced by those from yeast PSD1 both complemented the Etn requirement of a yeast psd1 psd2 mutant, and PSD activity was detected in the mitochondria of the complemented cells. Immunoblot analysis of potato (Solanum tuberosum) mitochondria demonstrated that PSD is located in mitochondrial membranes, and mRNA analysis in Arabidopsis showed that the mitochondrial PSD gene is expressed at low levels throughout the plant. An Arabidopsis knockup mutant grew normally but had 6- to 13-fold more mitochondrial PSD mRNA and 9-fold more mitochondrial PSD activity. Total membrane PSD activity was, however, unchanged in the mutant, showing mitochondrial activity to be a minor part of the total. These results establish that plants can synthesize Etn moieties via a phospholipid pathway and have both mitochondrial and extramitochondrial PSDs. They also indicate that mitochondrial PSD is an important housekeeping enzyme whose expression is strongly regulated at the transcriptional level.
机译:已知植物通过游离丝氨酸(Ser)的脱羧合成乙醇胺(Etn)部分,但是也有一些磷脂酰-Ser(Ptd-Ser)脱羧的证据。数据库搜索确定了多种植物cDNA和编码与酵母(Saccharomyces cerevisiae)和哺乳动物线粒体Ptd-Ser脱羧酶(PSDs)同源的50 kD蛋白的拟南芥基因。像后者一样,植物蛋白具有线粒体靶向作用和内膜分选序列,并且在C端附近含有一个Glycine-Serine-Threonine基序,对应于蛋白水解和催化丙酮酰残基形成的位置。缺少靶向序列的截短番茄(Lycopersicon esculentum)cDNA和嵌合构建体,其中靶向序列和排序序列被酵母PSD1的序列替代,均与酵母psd1 psd2突变体的Etn需求互补,并且在线粒体中检测到PSD活性补体细胞。马铃薯(Solanum tuberosum)线粒体的免疫印迹分析表明PSD位于线粒体膜上,而拟南芥中的mRNA分析表明线粒体PSD基因在整个植物中均以低水平表达。一个 拟南芥敲除突变体正常生长,但多了6至13倍 线粒体PSD mRNA和9倍以上的线粒体PSD活性。总 然而,该突变体的膜PSD活性没有变化,表明 线粒体活性仅占总数的一小部分。这些结果 建立植物可以通过磷脂途径合成Etn部分 并且具有线粒体和线粒体PSD。他们还表明 线粒体PSD是一种重要的管家酶,其表达为 在转录水平上受到严格调控。

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