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过氧化氢诱导大鼠离体主动脉反应性损伤:3-氨基-1,2,4-三唑的增强作用

Hydrogen peroxide-induced impairment of reactivity in rat isolated aorta: potentiation by 3-amino-1,2,4-triazole.

作者信息

Mian K B, Martin W

机构信息

Clinical Research Initiative, University of Glasgow.

出版信息

Br J Pharmacol. 1997 Jun;121(4):813-9. doi: 10.1038/sj.bjp.0701187.

Abstract
  1. In this study the impairment induced by hydrogen peroxide of vascular reactivity and the role of endogenous catalase in protection against this impairment was assessed in isolated rings of rat aorta. 2. Incubation with hydrogen peroxide at 1 mM, but not at 0.1 mM, for 15, 30 or 60 min followed by washout depressed, in a time-dependent manner, the subsequent ability of endothelium-containing and endothelium-denuded rings to contract to phenylephrine. 3. Incubation with 3-amino-1,2,4-triazole (50 mM, 90 min, followed by washout) to inhibit endogenous catalase had no effect by itself on subsequent phenylephrine-induced contraction. However, pretreatment with 3-amino-1,2,4-triazole did lead to a profound enhancement of the ability of hydrogen peroxide (1 mM, present for the final 30 min of the 90 min incubation, followed by washout) to depress phenylephrine-induced contraction in both endothelium-containing and endothelium-denuded rings. 4. Incubation with hydrogen peroxide at 1 mM, but not at 0.1 mM, for 15, 30 or 60 min followed by washout inhibited, in a time-dependent manner, the subsequent ability of acetylcholine (10 nM-3 microM) to induce endothelium-dependent relaxation. Furthermore, incubation with hydrogen peroxide 1 mM (30 min, followed by washout) also inhibited relaxation induced by glyceryl trinitrate (1-100 nM) or isoprenaline (10 nM-3 microM) in endothelium-denuded rings. 5. Incubation with 3-amino-1,2,4-triazole (50 mM, 90 min, followed by washout) had no effect by itself on relaxation induced by acetylcholine, glyceryl trinitrate or isoprenaline. In contrast, pretreatment with 3-amino-1,2,4-triazole led to profound enhancement of the ability of hydrogen peroxide (1 mM, present for final 30 min of the 90 min incubation) to block relaxation to acetylcholine, glyceryl trinitrate or isoprenaline. 6. On the basis of the actions of 3-amino-1,2,4-triazole, it is likely that endogenous catalase plays an important role in the protection of vascular reactivity of rat aorta against oxidant damage by high (1 mM) but not lower (0.1 mM) concentrations of hydrogen peroxide. The data are consistent with the promotion of non-selective damage to the vascular smooth muscle cells by hydrogen peroxide, but endothelial damage may also be sustained.
摘要
  1. 在本研究中,在大鼠主动脉离体环中评估了过氧化氢对血管反应性的损害以及内源性过氧化氢酶在抵御这种损害中的作用。2. 用1 mM过氧化氢孵育15、30或60分钟(而非0.1 mM),随后冲洗,会以时间依赖性方式降低含内皮环和去内皮环随后对去氧肾上腺素收缩的能力。3. 用3 - 氨基 - 1,2,4 - 三唑(50 mM,90分钟,随后冲洗)孵育以抑制内源性过氧化氢酶,其本身对随后去氧肾上腺素诱导的收缩没有影响。然而,用3 - 氨基 - 1,2,4 - 三唑预处理确实导致过氧化氢(1 mM,在90分钟孵育的最后30分钟存在,随后冲洗)降低含内皮环和去内皮环中去氧肾上腺素诱导收缩能力的作用显著增强。4. 用1 mM过氧化氢孵育15、30或60分钟(而非0.1 mM),随后冲洗,会以时间依赖性方式抑制乙酰胆碱(10 nM - 3 microM)随后诱导内皮依赖性舒张的能力。此外,用1 mM过氧化氢孵育(30分钟,随后冲洗)也抑制去内皮环中硝酸甘油(1 - 100 nM)或异丙肾上腺素(10 nM - 3 microM)诱导的舒张。5. 用3 - 氨基 - 1,2,4 - 三唑(50 mM,90分钟,随后冲洗)孵育,其本身对乙酰胆碱、硝酸甘油或异丙肾上腺素诱导的舒张没有影响。相反,用3 - 氨基 - 1,2,4 - 三唑预处理导致过氧化氢(1 mM,在90分钟孵育的最后30分钟存在)阻断对乙酰胆碱、硝酸甘油或异丙肾上腺素舒张能力的显著增强。6. 根据3 - 氨基 - 1,2,4 - 三唑的作用,内源性过氧化氢酶可能在保护大鼠主动脉血管反应性免受高浓度(1 mM)而非低浓度(0.1 mM)过氧化氢的氧化损伤中起重要作用。数据与过氧化氢对血管平滑肌细胞的非选择性损伤的促进作用一致,但也可能存在内皮损伤。

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