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首页> 外文期刊>Protoplasma: An International Journal of Cell Biology >MUTATIONAL ANALYSIS OF VAM4/YPT7P FUNCTION IN THE VACUOLAR BIOGENESIS AND MORPHOGENESIS IN THE YEAST, SACCHAROMYCES CEREVISIAE
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MUTATIONAL ANALYSIS OF VAM4/YPT7P FUNCTION IN THE VACUOLAR BIOGENESIS AND MORPHOGENESIS IN THE YEAST, SACCHAROMYCES CEREVISIAE

机译:VAM4 / YPT7P功能在酵母,酿酒酵母中的肺泡形成和形态发生中的突变分析

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摘要

The vacuole is one of the most prominent compartments in yeast cells. The wild-type yeast cells have a large vacuolar compartment which occupies approximately a quarter of the cell volume, while the vam4 mutant cells exhibit highly fragmented vacuolar morphology. We isolated the VAM4 gene and found that the VAM4 is identical to the YPT7 which encodes a member of small GTP-binding protein superfamily. We introduced mutations to the VAM4/YPT7 which alter nucleotide binding characteristics of the gene product specifically, and their activities for the vacuolar morphogenesis were examined by transforming the mutant genes into yeast cells. The Thr22Asn mutation, which was expected to fix the protein in the GDP-bound state, resulted in loss of function in the vacuolar morphogenesis. Subcellular fractionation analysis indicated that the mutant molecule did nor associate with intracellular membranes efficiently. In contrast, Vam4/Ypt7p with the Gln68Leu mutation, which was expected to be the GTP-bound form, complemented the fragmented vacuolar morphology of Delta vam4 mutant cells. Vam4/Ypt7p with the Gln68Leu mutation also complemented the defects in the biogenesis of vacuolar alkaline phosphatase whose maturation requires the proper function of Vam4/Ypt7p. Overexpression of the mutant proteins in wild-type cells did not develop dominant-negative effects on the vacuolar assembly. These results indicated that the GTP-bound form of Vam4/Ypt7p promotes the biogenesis and morphogenesis of the yeast vacuolar compartment. [References: 37]
机译:液泡是酵母细胞中最突出的区室之一。野生型酵母细胞具有较大的液泡区室,约占细胞体积的四分之一,而vam4突变细胞显示出高度碎片化的液泡形态。我们分离了VAM4基因,发现VAM4与YPT7相同,后者编码小GTP结合蛋白超家族的成员。我们向VAM4 / YPT7引入了可特异性改变基因产物核苷酸结合特性的突变,并通过将突变基因转化为酵母细胞来检查了它们对液泡形态发生的活性。 Thr22Asn突变有望将蛋白质固定在GDP结合状态,导致液泡形态发生功能丧失。亚细胞分级分析表明该突变分子也没有有效地与细胞内膜结合。相比之下,具有Gln68Leu突变的Vam4 / Ypt7p被认为是GTP结合形式,与Delta vam4突变细胞的碎片状液泡形态互补。具有Gln68Leu突变的Vam4 / Ypt7p也弥补了液泡碱性磷酸酶的生物发生缺陷,后者成熟需要Vam4 / Ypt7p的适当功能。在野生型细胞中突变蛋白的过表达对液泡组装没有显性的负作用。这些结果表明,Vam4 / Ypt7p的GTP结合形式促进了酵母液泡区室的生物发生和形态发生。 [参考:37]

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