Li Y, Trush M A, Yager J D
Department of Environmental Health Sciences, Johns Hopkins University School of Hygiene and Public Health, Baltimore, MD 21205.
Carcinogenesis. 1994 Jul;15(7):1421-7. doi: 10.1093/carcin/15.7.1421.
It has previously been proposed that redox cycling between catechol estrogens and their quinones, mediated by cytochrome P450, could lead to the generation of free radicals that would subsequently cause oxidative damage to DNA and proteins that might have a role in hormonal carcinogenesis. Alternative, non-enzymatic mechanisms involving copper have been shown to participate in the oxidation of various chemicals through processes that also result in the appearance of reactive oxygen species and subsequent site-specific oxidative DNA damage. The goal of the present study was to determine whether the 2-hydroxy-catechol of estradiol (2-OH-E2) can be oxidized by copper through a process which generates reactive oxygen species that cause oxidative DNA damage as detected by the appearance of strand breaks in phi X-174 plasmid DNA. Our results show that both single- and double-strand breaks are formed in the presence of Cu(II) plus micromolar concentrations of 2-OH-E2, and 4-OH-E2, in a concentration/time-dependent process. No strand breaks were detected in the presence of Cu(II) or 2-OH-E2 alone. The reaction of 2-OH-E2 with Cu(II) was accompanied by the reduction of Cu(II) to Cu(I), the utilization of O2, and the generation of H2O2. The utilization of O2 and the formation of strand breaks was completely blocked by the Cu(I)-specific chelator bathocuproinedisulfonic acid (BCS) at a ratio of BCS to Cu(II) of 4:1. The appearance of strand breaks was also blocked by catalase and inhibited by the singlet oxygen scavengers sodium azide and 2,2,6,6-tetramethyl-4-piperidone. In contrast the free hydroxyl radical scavengers mannitol and N-tert-butyl-alpha-phenylnitrone were not effective inhibitors; superoxide dismutase had no inhibitory effect. These results are similar to what has been observed by others for the formation of oxidative DNA damage by the H2O2/Cu(II) system and by us for the induction of strand breaks by hydroquinone/Cu(II). Since copper is known to be present in the nucleus, particularly in association with guanines in DNA, our results with 2-OH-E2/Cu(II) together with those of others with H2O2/Cu(II), discussed below, suggest an alternate site-specific mechanism for the formation of oxidative DNA damage associated with estrogen treatment. Furthermore, the results suggest that the oxidative damage results from the localized generation of singlet oxygen or a similar bound reactive entity rather than free hydroxyl radical.
先前有人提出,由细胞色素P450介导的儿茶酚雌激素与其醌之间的氧化还原循环,可能导致自由基的产生,进而对DNA和蛋白质造成氧化损伤,这可能在激素致癌过程中发挥作用。已表明涉及铜的非酶替代机制通过同样导致活性氧出现及随后位点特异性氧化DNA损伤的过程,参与各种化学物质的氧化。本研究的目的是确定雌二醇的2-羟基儿茶酚(2-OH-E2)是否能被铜氧化,该过程会产生活性氧,通过检测phi X-174质粒DNA中的链断裂来确定是否会导致氧化DNA损伤。我们的结果表明,在Cu(II)加上微摩尔浓度的2-OH-E2和4-OH-E2存在的情况下,单链和双链断裂均以浓度/时间依赖性过程形成。单独存在Cu(II)或2-OH-E2时未检测到链断裂。2-OH-E2与Cu(II)的反应伴随着Cu(II)还原为Cu(I)、O2的消耗以及H2O2的产生。O2的消耗和链断裂的形成在Cu(I)特异性螯合剂 bathocuproinedisulfonic acid(BCS)以BCS与Cu(II) 4:1的比例存在时被完全阻断。链断裂的出现也被过氧化氢酶阻断,并被单线态氧清除剂叠氮化钠和2,2,6,6-四甲基-4-哌啶酮抑制。相比之下,游离羟基自由基清除剂甘露醇和N-叔丁基-α-苯基硝酮不是有效的抑制剂;超氧化物歧化酶没有抑制作用。这些结果与其他人观察到的H2O2/Cu(II)系统形成氧化DNA损伤以及我们观察到的对苯二酚/Cu(II)诱导链断裂的结果相似。由于已知铜存在于细胞核中,特别是与DNA中的鸟嘌呤结合,我们用2-OH-E2/Cu(II)得到的结果以及其他人用H2O2/Cu(II)得到的结果(如下所述)表明,雌激素治疗相关的氧化DNA损伤形成存在另一种位点特异性机制。此外,结果表明氧化损伤是由单线态氧或类似的结合反应性实体的局部产生而非游离羟基自由基导致的。
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