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The Pbs2 MAP kinase kinase is essential for the oxidative-stress response in the fungal pathogen Candida albicans

机译:PBS2映射激酶激酶对于真菌病原体念珠菌蛋白糖苷中的氧化应激反应是必不可少的

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The human fungal pathogen Candida albicans responds to stress by phosphorylation of the Hog1 MAP kinase. PBS2 was cloned and shown to encode the MAP kinase kinase that is involved in this activation, as determined by immunoblot analyses using antibodies that recognize the active form of the target Hog1 protein. Characterization of pbs2 mutants revealed that they were sensitive to both osmotic and oxidative stress and that they, interestingly, displayed differential behaviour from that of hog1 mutants, losing viability when exposed to an oxidative challenge more rapidly than the hog1 strain. Hog1 and Pbs2 were also shown to be involved in the mechanism of adaptation to oxidative stress, as evidenced by the enhanced susceptibility to oxidants of pbs2 and hog1 mutants, compared with the wild-type strain, when cells were previously exposed to a low, sub-lethal concentration of hydrogen peroxide and by the PBS2-dependent diminished activation of Hog1 MAP kinase in the adaptive process. Studies with a chimaeric Hog1–green fluorescent protein fusion revealed that this protein was localized throughout the cell (being excluded from the vacuole), but concentrated in the nucleus in response to NaCl stress, a process that was dependent on the Pbs2 protein. Both Hog1 and Pbs2 also play a role in controlling the phosphorylation state of the other MAP kinases Mkc1 and Cek1, involved respectively in cell-wall integrity and invasive growth. Furthermore, it is demonstrated that PBS2 plays a role in cell-wall biogenesis in this fungal pathogen, as its deletion renders cells with an altered susceptibility to certain cell wall-interfering compounds.
机译:人类真菌病原体念珠菌蛋白白醛糖酸响应猪映射激酶磷酸化的应力。克隆PBS2并显示编码参与该活化的地图激酶激酶,如使用识别靶猪蛋白的活性形式的抗体的免疫印迹分析所确定的。 PBS2突变体的表征揭示它们对渗透和氧化应激敏感,并且有趣的是,从霍夫1突变体的差异表现出差异行为,在暴露于氧化攻击时比霍格1菌株更快地失去活力。还显示出猪和PBS2参与适应于氧化应激的机制,与PBS2和Hog1突变体的氧化剂的易感性增强,与野生型菌株相比,当细胞预先暴露于低电平 - 在自适应过程中,通过过氧化氢的浓度和PBS2依赖性减少活化的肝脏映射激酶的激活。用Chimaeric Hog1-Green荧光蛋白融合的研究表明,该蛋白质在整个细胞中定位(被排除在液泡之外),但响应于NaCl应力浓缩在核中,该方法依赖于PBS2蛋白。 Hog1和PBS2也在控制分别参与细胞壁完整性和侵入性生长的其他地图激酶MKC1和CEK1的磷酸化状态方面发挥作用。此外,证明PBS2在该真菌病原体中起着在细胞壁生物发生中起作用,因为其缺失使细胞具有改变对某些细胞壁干扰化合物的易感性。

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