Dept. of Physiology, Medical College of Wisconsin, 8701 Watertown Plank Rd., Milwaukee, WI 53226, USA.
Am J Physiol Renal Physiol. 2012 Jan 1;302(1):F95-F102. doi: 10.1152/ajprenal.00469.2011. Epub 2011 Oct 5.
The mitochondria-rich epithelial cells of the renal medullary thick ascending limb (mTAL) reabsorb nearly 25% of filtered sodium (Na(+)) and are a major source of cellular reactive oxygen species. Although we have shown that delivery of Na(+) to the mTAL of rats increases superoxide (O(2)(·-)) production in mTAL, little is known about H(2)O(2) production, given the lack of robust and selective fluorescent indicators for determining changes within the whole cell, specifically in the mitochondria. The present study determined the effect of increased tubular flow and Na(+) delivery to mTAL on the production of mitochondrial H(2)O(2) in mTAL. H(2)O(2) responses were determined in isolated, perfused mTAL of Sprague-Dawley rats using a novel mitochondrial selective fluorescent H(2)O(2) indicator, mitochondria peroxy yellow 1, and a novel, highly sensitive and stable cytosolic-localized H(2)O(2) indicator, peroxyfluor-6 acetoxymethyl ester. The results showed that mitochondrial H(2)O(2) and cellular fluorescent signals increased progressively over a period of 30 min following increased tubular perfusion (5-20 nl/min), reaching levels of statistical significance at ∼10-12 min. Responses were inhibited with rotenone or antimycin A (inhibitors of the electron-transport chain), polyethylene glycol-catalase and by reducing Na(+) transport with furosemide or ouabain. Inhibition of membrane NADPH-oxidase with apocynin had no effect on mitochondrial H(2)O(2) production. Cytoplasmic H(2)O(2) (peroxyfluor-6 acetoxymethyl ester) increased in parallel with mitochondrial H(2)O(2) (mitochondria peroxy yellow 1) and was partially attenuated (∼65%) by rotenone and completely inhibited by apocynin. The present data provide clear evidence that H(2)O(2) is produced in the mitochondria in response to increased flow and delivery of Na(+) to the mTAL, and that whole cell H(2)O(2) levels are triggered by the mitochondrial reactive oxygen species production. The mitochondrial production of H(2)O(2) may represent an important target for development of more effective antioxidant therapies.
肾髓质升支粗段(mTAL)富含线粒体的上皮细胞重吸收近 25%的滤过钠(Na(+)),是细胞活性氧物质的主要来源。尽管我们已经表明,向大鼠 mTAL 输送 Na(+)会增加 mTAL 中超氧阴离子(O(2)(·-))的产生,但由于缺乏用于确定整个细胞内(特别是在线粒体中)变化的稳健和选择性荧光指示剂,因此对于 H(2)O(2)的产生知之甚少。本研究确定了增加管状流量和 Na(+)向 mTAL 输送对 mTAL 中线粒体 H(2)O(2)产生的影响。使用新型线粒体选择性荧光 H(2)O(2)指示剂线粒体过氧黄 1 和新型、高度敏感和稳定的胞质 H(2)O(2)指示剂过氧氟-6 乙酰氧甲酯,在分离灌注的 Sprague-Dawley 大鼠 mTAL 中确定 H(2)O(2)反应。结果表明,在增加管状灌注(5-20 nl/min)后的 30 分钟内,线粒体 H(2)O(2)和细胞荧光信号逐渐增加,在约 10-12 分钟达到统计学显著水平。用鱼藤酮或抗霉素 A(电子传递链抑制剂)、聚乙二醇-过氧化氢酶和用呋塞米或哇巴因减少 Na(+)转运抑制反应。用 apocynin 抑制膜 NADPH-氧化酶对线粒体 H(2)O(2)的产生没有影响。细胞质 H(2)O(2)(过氧氟-6 乙酰氧甲酯)与线粒体 H(2)O(2)(线粒体过氧黄 1)平行增加,被鱼藤酮部分减弱(约 65%),并被 apocynin 完全抑制。本数据提供了明确的证据,表明 H(2)O(2)是在响应增加的 mTAL 中 Na(+)的流量和输送而在线粒体中产生的,并且整个细胞 H(2)O(2)水平是由线粒体活性氧物质的产生触发的。H(2)O(2)的线粒体产生可能代表开发更有效的抗氧化治疗方法的重要目标。
