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双嘧达莫和RA - 642可抑制超氧阴离子的产生以及对大鼠晶状体的自由基损伤。

Dipyridamole and RA-642 inhibit the production of superoxide anion and free radical damage to rat lens.

作者信息

De la Cruz J P, Sintas A, Moreno A, Garcia-Campos J, Sanchez de la Cuesta F

机构信息

Department of Pharmacology and Therapeutics, School of Medicine, University of Málaga, Spain.

出版信息

Pharmacol Toxicol. 1991 Sep;69(3):201-4. doi: 10.1111/j.1600-0773.1991.tb01297.x.

Abstract

We studied the effects of dipyridamole and RA-642 on the production of superoxide anions and on oxygen radicals-induced lipid peroxidation in lens tissue homogenates from normal rats and rats given dipyridamole or RA-642 intraperitoneally. Superoxide production was evaluated by phenazine methosulphate (PMS)-induced nitroblue tetrazolium (NBT) reduction and lipid peroxidation by ferrous sulfate and ascorbic acid (FeAs)-induced malondialdehyde (MDA) production. Dipyridamole and RA-642 showed an inhibitory effect on both assays in the experiments with lens tissue homogenates from untreated or treated rats. The extent of inhibition, however, was significantly higher in pyrimidopyrimidinic-treated rats (range of inhibition at different times of incubation was 18% versus 23-57% for dipyridamole and 14% versus 73-80% for RA-642 in the assay of MDA production, and 10% versus 33-37% for dipyridamole and 2.5% versus 11-32% for RA-642 in the assay of NBT reduction). Concentrations of dipyridamole and RA-642 in lens tissue from treated animals could not be determined (less than 0.001 micrograms/mg of tissue). Although both compounds inhibited lipid peroxidation induced by oxygen free radicals, the mechanism of action might include the role of adenosine as a mediator.

摘要

我们研究了双嘧达莫和RA-642对正常大鼠以及腹腔注射双嘧达莫或RA-642的大鼠晶状体组织匀浆中超氧阴离子生成及氧自由基诱导的脂质过氧化的影响。通过吩嗪硫酸甲酯(PMS)诱导的硝基蓝四唑(NBT)还原评估超氧阴离子生成,通过硫酸亚铁和抗坏血酸(FeAs)诱导的丙二醛(MDA)生成评估脂质过氧化。在未处理或已处理大鼠的晶状体组织匀浆实验中,双嘧达莫和RA-642在两种检测中均显示出抑制作用。然而,在嘧啶并嘧啶处理的大鼠中,抑制程度明显更高(在MDA生成检测中,双嘧达莫在不同孵育时间的抑制范围为18%,而RA-642为23%-57%;在NBT还原检测中,双嘧达莫为10%,而RA-642为2.5%-11%-32%)。无法测定处理动物晶状体组织中双嘧达莫和RA-642的浓度(低于0.001微克/毫克组织)。尽管两种化合物均抑制氧自由基诱导的脂质过氧化,但其作用机制可能包括腺苷作为介质的作用。

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