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首页> 外文期刊>Biochimica et biophysica acta. Molecular cell research >Saccharomyces cerevisiae cells lacking Pex3 contain membrane vesicles that harbor a subset of peroxisomal membrane proteins
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Saccharomyces cerevisiae cells lacking Pex3 contain membrane vesicles that harbor a subset of peroxisomal membrane proteins

机译:缺乏Pex3的酿酒酵母细胞含有膜囊泡,含有过氧甲虫膜蛋白的子集

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摘要

Abstract Pex3 has been proposed to be important for the exit of peroxisomal membrane proteins (PMPs) from the ER, based on the observation that PMPs accumulate at the ER in Saccharomyces cerevisiae pex3 mutant cells. Using a combination of microscopy and biochemical approaches, we show that a subset of the PMPs, including the receptor docking protein Pex14, localizes to membrane vesicles in S. cerevisiae pex3 cells. These vesicles are morphologically distinct from the ER and do not co-sediment with ER markers in cell fractionation experiments. At the vesicles, Pex14 assembles with other peroxins (Pex13, Pex17, and Pex5) to form a complex with a composition similar to the PTS1 import pore in wild-type cells. Fluorescence microscopy studies revealed that also the PTS2 receptor Pex7, the importomer organizing peroxin Pex8, the ubiquitin conjugating enzyme Pex4 with its recruiting PMP Pex22, as well as Pex15 and Pex25 co-localize with Pex14. Other peroxins (including the RING finger complex and Pex27) did not accumulate at these structures, of which Pex11 localized to mitochondria. In line with these observations, proteomic analysis showed that in addition to the docking proteins and Pex5, also Pex7, Pex4/Pex22 and Pex25 were present in Pex14 complexes isolated from pex3 cells. However, formation of the entire importomer was not observed, most likely because Pex8 and the RING proteins were absent in the Pex14 protein complexes. Our data suggest that peroxisomal membrane vesicles can form in the absence of Pex3 and that several PMPs can insert in these vesicles in a Pex3 independent manner. Highlights ? Peroxisomal membrane vesicles exist in Saccharomyces cerevisiae pex3 cells. ? Peroxisomal membrane proteins do not accumulate at the ER in yeast pex3 cells. ? In the absence of Pex3 the PTS1 import pore can be formed. ? Only a subset of the peroxisomal membrane proteins are missorted in pex3 cells. ]]>
机译:摘要已经提出了PEX3对于从ER的过氧敏血膜蛋白(PMP)出口是重要的,所述观察PMP在酿酒酵母群突变细胞中的ER中积聚在ER中。使用显微镜和生物化学方法的组合,我们表明PMP的子集,包括受体对接蛋白PEX14,定位于酿酒酵母PEX3细胞中的膜囊泡。这些囊泡在形态上与ER不同,并且不与细胞分级实验中的ER标记共沉淀。在囊泡中,Pex14与其他过氧化物(Pex13,Pex17和Pex5)组合,形成与野生型电池中的PTS1进口孔相似的组合物。荧光显微镜研究表明,除了用募集PMP Pex22以及Pex15和Pex25与Pex14共定位,也表明PTS2受体Pex7,泛素缀合物酶Pex4和Pex15和Pex25共定为Pex14的PTS2受体Pex7。其他过氧化物(包括环手指复合物和Pex27)在这些结构上没有积聚,其中PEX11本地化为线粒体。符合这些观察结果,蛋白质组学分析表明,除了对接蛋白和Pex5之外,Pex7,Pex4 / Pex22和Pex25还存在于从Pex3细胞分离的Pex14复合物中存在。然而,未观察到整个进化器的形成,最有可能因为在PEX14蛋白络合物中不存在PEX8和环蛋白。我们的数据表明,过氧化物膜囊泡可以在没有PEX3的情况下形成,并且几个PMP可以以PEX3独立的方式插入这些囊泡中。强调 ?过氧甲基乙烯膜囊泡存在于酿酒酵母中PEX3细胞。还过氧化物膜蛋白在酵母Pex3细胞中不会在ER中积聚。还在没有PEX3的情况下,可以形成PTS1进口孔隙。还仅在Pex3细胞中仅在过氧血清膜蛋白的子集中进行。 ]]>

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