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Cellular Redox State Acts as Switch to Determine the Direction of NNT-Catalyzed Reaction in Cystic Fibrosis Cells

机译:细胞氧化还原状态充当开关以确定囊性纤维化细胞中NNT催化反应的方向

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摘要

The redox states of NAD and NADP are linked to each other in the mitochondria thanks to the enzyme nicotinamide nucleotide transhydrogenase (NNT) which, by utilizing the mitochondrial membrane potential (mΔΨ), catalyzes the transfer of redox potential between these two coenzymes, reducing one at the expense of the oxidation of the other. In order to define NNT reaction direction in CF cells, NNT activity under different redox states of cell has been investigated. Using spectrophotometric and western blotting techniques, the presence, abundance and activity level of NNT were determined. In parallel, the levels of NADPH and NADH as well as of mitochondrial and cellular ROS were also quantified. CF cells showed a 70% increase in protein expression compared to the Wt sample; however, regarding NNT activity, it was surprisingly lower in CF cells than healthy cells (about 30%). The cellular redox state, together with the low mΔΨ, pushes to drive NNT reverse reaction, at the expense of its antioxidant potential, thus consuming NADPH to support NADH production. At the same time, the reduced NNT activity prevents the NADH, produced by the reaction, from causing an explosion of ROS by the damaged respiratory chain, in accordance with the reduced level of mitochondrial ROS in NNT-loss cells. This new information on cellular bioenergetics represents an important building block for further understanding the molecular mechanisms responsible for cellular dysfunction in cystic fibrosis.
机译:由于酶烟酰胺核苷酸转氢酶(NNT),NAD和NADP的氧化还原态在线粒体中彼此联系,这通过利用线粒体膜电位(MΔΣ),催化在这两种辅酶之间的氧化还原电位的转移,减少一个以牺牲对方的氧化。为了在CF细胞中定义NNT反应方向,已经研究了不同氧化还原态下的NNT活性。使用分光光度和蛋白质印迹技术,测定NNT的存在,丰度和活性水平。平行,NADPH和NADH以及线粒体和细胞RO的水平也被定量。与WT样品相比,CF细胞显示蛋白质表达增加70%;然而,关于NNT活性,CF细胞中令人惊讶地低于健康细胞(约30%)。细胞氧化还原状态与低Mδ1一起推动以牺牲其抗氧化潜力的牺牲逆反应驱动NNT反应,从而消耗NADPH以支持NADH生产。同时,减少的NNT活性可防止由反应产生的NADH,从导致损伤的呼吸链爆炸,根据NNT-损失细胞中的线粒体RO的降低。关于细胞生物植物学的新信息代表了一个重要的构建块,用于进一步了解负责细胞功能障碍在囊性纤维化中的分子机制。

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