首页> 美国卫生研究院文献>The Plant Cell >The Arabidopsis thaliana Type I Isopentenyl Diphosphate Isomerases Are Targeted to Multiple Subcellular Compartments and Have Overlapping Functions in Isoprenoid Biosynthesis
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The Arabidopsis thaliana Type I Isopentenyl Diphosphate Isomerases Are Targeted to Multiple Subcellular Compartments and Have Overlapping Functions in Isoprenoid Biosynthesis

机译:拟南芥I型异戊烯基二磷酸异构酶是针对多个亚细胞隔室并在类异戊二烯生物合成中具有重叠功能

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摘要

To form the building blocks of isoprenoids, isopentenyl diphosphate (IPP) isomerase activity, which converts IPP to dimethylallyl diphosphate (DMAPP), appears to be necessary in cytosol, plastids, and mitochondria. Arabidopsis thaliana contains only two IPP isomerases (Isopentenyl Diphosphate Isomerase1 [IDI1] and IDI2). Both encode proteins with N-terminal extensions similar to transit peptides and are expressed in all organs, with IDI1 less abundant than IDI2. Examination of enhanced green fluorescent protein fusions established that IDI1 is mainly in the plastid, whereas IDI2 is mainly in the mitochondria. Both proteins are also in the cytosol as a result of their translation from naturally occurring shorter transcripts lacking transit peptides, as demonstrated by 5′ rapid amplification of cDNA ends cloning. IPP isomerase activity in the cytosol was confirmed by uniform labeling of IPP- and DMAPP-derived units of the cytoplasmic isoprenoid product, sitosterol, when labeled mevalonate was administered. Analysis of mutant lines showed that double mutants were nonviable, while homozygous single mutants had no major morphological or chemical differences from the wild type except for flowers with fused sepals and underdeveloped petals on idi2 mutants. Thus, each of the two Arabidopsis IPP isomerases is found in multiple but partially overlapping subcellular locations, and each can compensate for the loss of the other through partial redundancy in the cytosol.
机译:为了形成类异戊二烯的组成部分,将异戊烯二磷酸(IPP)异构酶活性(将IPP转换为二甲基烯丙基二磷酸酯(DMAPP))似乎在细胞质,质体和线粒体中都是必需的。拟南芥仅包含两种IPP异构酶(异戊烯基二磷酸异构酶1 [IDI1]和IDI2)。两者都编码具有类似于转运肽的N端延伸的蛋白质,并且在所有器官中都有表达,IDI1的丰度低于IDI2。增强的绿色荧光蛋白融合体的检查确定IDI1主要在质体中,而IDI2主要在线粒体中。两种蛋白质都因其从缺乏转运肽的天然存在的较短转录物的翻译而在胞质溶胶中,如cDNA末端克隆的5'快速扩增所证明的。当给予标记的甲羟戊酸酯时,通过对IPP和DMAPP衍生的胞质类异戊二烯产品谷固醇的单位进行统一标记,可以确认胞质溶胶中的IPP异构酶活性。突变株系的分析表明,双重突变株是不可行的,而纯合的单个突变株与野生型相比没有主要的形态或化学差异,除了在idi2突变株上具有融合的萼片和不发达的花瓣的花。因此,两个拟南芥IPP异构酶中的每一个都存在于多个但部分重叠的亚细胞位置,并且每个都可以通过胞浆中的部分冗余来补偿另一个的损失。

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