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超氧阴离子调节小鼠入球小动脉的肌源性收缩。

Superoxide modulates myogenic contractions of mouse afferent arterioles.

机构信息

Division of Nephrology and Hypertension, Georgetown University, Washington, DC 20007, USA.

出版信息

Hypertension. 2011 Oct;58(4):650-6. doi: 10.1161/HYPERTENSIONAHA.111.170472. Epub 2011 Aug 22.

DOI:10.1161/HYPERTENSIONAHA.111.170472
PMID:21859962
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3190586/
Abstract

Reactive oxygen species enhance or impair autoregulation. Because superoxide is a vasoconstrictor, we tested the hypothesis that stretch generates superoxide that mediates myogenic responses. Increasing perfusion pressure of mouse isolated perfused renal afferent arterioles from 40 to 80 mm Hg reduced their diameter by 13.3±1.8% (P<0.001) and increased reactive oxygen species (ethidium: dihydroethidium fluorescence) by 9.8±2.3% (P<0.05). Stretch-induced fluorescence was reduced significantly (P<0.05) by incubation with Tempol (3.7±0.8%), pegylated superoxide dismutase (3.2±1.0%), or apocynin (3.5±0.9%) but not by pegylated catalase, L-nitroarginine methylester, or Ca(2+)-free medium, relating it to Ca(2+)-independent vascular superoxide. Compared with vehicle, basal tone and myogenic contractions were reduced significantly (P<0.05) by pegylated superoxide dismutase (5.4±0.8), Tempol (4.1±1.0%), apocynin (1.0±1.3%), and diphenyleneiodinium (3.9±0.9%) but not by pegylated catalase (10.1±1.6%). L-Nitroarginine methylester enhanced basal tone, but neither it (15.8±3.3%) nor endothelial NO synthase knockout (10.2±1.8%) significantly changed myogenic contractions. Tempol had no further effect after superoxide dismutase but remained effective after catalase. H(2)O(2) >50 μmol/L caused contractions but at 25 μmol/L inhibited myogenic responses (7.4±0.8%; P<0.01). In conclusion, increasing the pressure within afferent arterioles led to Ca(2+)-independent increased vascular superoxide production from nicotinamide adenine dinucleotide phosphate oxidase, which enhanced myogenic contractions largely independent of NO, whereas H(2)O(2) impaired pressure-induced contractions but was not implicated in the normal myogenic response.

摘要

活性氧增强或损害自身调节。由于超氧化物是血管收缩剂,我们测试了这样的假设,即牵张产生超氧化物,介导肌源性反应。将小鼠离体灌注肾传入小动脉的灌注压从 40mmHg 增加到 80mmHg,可使小动脉直径减少 13.3±1.8%(P<0.001),并使活性氧(ethidium:dihydroethidium 荧光)增加 9.8±2.3%(P<0.05)。孵育 Tempol(3.7±0.8%)、聚乙二醇化超氧化物歧化酶(3.2±1.0%)或 apocynin(3.5±0.9%)可显著降低牵张诱导的荧光(P<0.05),但聚乙二醇化过氧化氢酶、L-硝基精氨酸甲酯或无钙培养基不影响其荧光,提示与 Ca2+非依赖性血管超氧化物有关。与载体相比,聚乙二醇化超氧化物歧化酶(5.4±0.8)、Tempol(4.1±1.0)、apocynin(1.0±1.3)和二苯碘(3.9±0.9)显著降低基础张力和肌源性收缩(P<0.05),但聚乙二醇化过氧化氢酶(10.1±1.6)无影响。L-硝基精氨酸甲酯增强基础张力,但内皮型一氧化氮合酶敲除(10.2±1.8%)或其不影响肌源性收缩。超氧化物歧化酶后 Tempol 无进一步作用,但过氧化氢酶后仍有效。H2O2>50μmol/L 引起收缩,但 25μmol/L 抑制肌源性反应(7.4±0.8%;P<0.01)。总之,增加传入小动脉的压力导致 NADPH 氧化酶产生 Ca2+非依赖性血管超氧化物增加,这大大增强了肌源性收缩,而 NO 则不参与;而 H2O2 损害压力诱导的收缩,但不参与正常的肌源性反应。

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