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巴斯德毕赤酵母PAS1基因在过氧化物酶体生物发生中的作用。

Role of the PAS1 gene of Pichia pastoris in peroxisome biogenesis.

作者信息

Heyman J A, Monosov E, Subramani S

机构信息

Department of Biology, University of California, San Diego, La Jolla 92093-0322.

出版信息

J Cell Biol. 1994 Dec;127(5):1259-73. doi: 10.1083/jcb.127.5.1259.

Abstract

Several groups have reported the cloning and sequencing of genes involved in the biogenesis of yeast peroxisomes. Yeast strains bearing mutations in these genes are unable to grow on carbon sources whose metabolism requires peroxisomes, and these strains lack morphologically normal peroxisomes. We report the cloning of Pichia pastoris PAS1, the homologue (based on a high level of protein sequence similarity) of the Saccharomyces cerevisiae PAS1. We also describe the creation and characterization of P. pastoris pas1 strains. Electron microscopy on the P. pastoris pas1 cells revealed that they lack morphologically normal peroxisomes, and instead contain membrane-bound structures that appear to be small, mutant peroxisomes, or "peroxisome ghosts." These "ghosts" proliferated in response to induction on peroxisome-requiring carbon sources (oleic acid and methanol), and they were distributed to daughter cells. Biochemical analysis of cell lysates revealed that peroxisomal proteins are induced normally in pas1 cells. Peroxisome ghosts from pas1 cells were purified on sucrose gradients, and biochemical analysis showed that these ghosts, while lacking several peroxisomal proteins, did import varying amounts of several other peroxisomal proteins. The existence of detectable peroxisome ghosts in P. pastoris pas1 cells, and their ability to import some proteins, stands in contrast with the results reported by Erdmann et al. (1991) for the S. cerevisiae pas1 mutant, in which they were unable to detect peroxisome-like structures. We discuss the role of PAS1 in peroxisome biogenesis in light of the new information regarding peroxisome ghosts in pas1 cells.

摘要

几个研究小组报道了参与酵母过氧化物酶体生物合成的基因的克隆和测序。在这些基因中携带突变的酵母菌株无法在其代谢需要过氧化物酶体的碳源上生长,并且这些菌株缺乏形态正常的过氧化物酶体。我们报道了巴斯德毕赤酵母PAS1的克隆,它是酿酒酵母PAS1的同源物(基于高度的蛋白质序列相似性)。我们还描述了巴斯德毕赤酵母pas1菌株的构建和特性。对巴斯德毕赤酵母pas1细胞的电子显微镜观察显示,它们缺乏形态正常的过氧化物酶体,取而代之的是含有似乎是小的、突变的过氧化物酶体或“过氧化物酶体空壳”的膜结合结构。这些“空壳”在需要过氧化物酶体的碳源(油酸和甲醇)诱导下增殖,并分布到子细胞中。对细胞裂解物的生化分析表明,过氧化物酶体蛋白在pas1细胞中正常诱导。来自pas1细胞的过氧化物酶体空壳在蔗糖梯度上进行纯化,生化分析表明,这些空壳虽然缺乏几种过氧化物酶体蛋白,但确实导入了不同量的其他几种过氧化物酶体蛋白。巴斯德毕赤酵母pas1细胞中可检测到过氧化物酶体空壳的存在及其导入一些蛋白质的能力,与埃德曼等人(1991年)报道的酿酒酵母pas1突变体的结果形成对比,在该突变体中他们无法检测到过氧化物酶体样结构。我们根据关于pas1细胞中过氧化物酶体空壳的新信息讨论了PAS1在过氧化物酶体生物合成中的作用。

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