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Genes Required for Vacuolar Acidity in Saccharomyces Cerevisiae

机译:酿酒酵母液泡酸度所需的基因

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摘要

Mutations that cause loss of acidity in the vacuole (lysosome) of Saccharomyces cerevisiae were identified by screening colonies labeled with the fluorescent, pH-sensitive, vacuolar labeling agent, 6-carboxyfluorescein. Thirty nine vacuolar pH (Vph(-)) mutants were identified. Four of these contained mutant alleles of the previously described PEP3, PEP5, PEP6 and PEP7 genes. The remaining mutants defined eight complementation groups of vph mutations. No alleles of the VAT2 or TFP1 genes (known to encode subunits of the vacuolar H(+)-ATPase) were identified in the Vph(-) screen. Strains bearing mutations in any of six of the VPH genes failed to grow on medium buffered at neutral pH; otherwise, none of the vph mutations caused notable growth inhibition on standard yeast media. Expression of the vacuolar protease, carboxypeptidase Y, was defective in strains bearing vph4 mutations but was apparently normal in strains bearing any of the other vph mutations. Defects in vacuolar morphology at the light microscope level were evident in all Vph(-) mutants. Strains that contained representative mutant alleles of the 17 previously described PEP genes were assayed for vacuolar pH; mutations in seven of the PEP genes (including PEP3, PEP5, PEP6 and PEP7) caused loss of vacuolar acidity.
机译:通过筛选用荧光,pH敏感,液泡标记剂6-羧基荧光素标记的菌落,鉴定出导致酿酒酵母液泡(溶酶体)中酸度损失的突变。确定了39个液泡pH(Vph(-))突变体。这些中的四个包含先前描述的PEP3,PEP5,PEP6和PEP7基因的突变等位基因。其余的突变体定义了vph突变的八个互补组。在Vph(-)筛选中未发现VAT2或TFP1基因的等位基因(已知编码液泡H(+)-ATPase的亚基)。在中性pH缓冲的培养基上,不能在六个VPH基因中的任何一个上携带突变的菌株。否则,没有任何vph突变引起对标准酵母培养基的明显生长抑制。液泡蛋白酶羧肽酶Y的表达在带有vph4突变的菌株中是有缺陷的,但是在带有任何其他vph突变的菌株中显然是正常的。在所有Vph(-)突变体中,在光学显微镜下液泡形态的缺陷均很明显。分析含有17个先前描述的PEP基因的代表性突变等位基因的菌株的液泡pH; 7个PEP基因(包括PEP3,PEP5,PEP6和PEP7)的突变导致液泡酸度降低。

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