耗尽谷胱甘肽水平对CHO K1细胞中酞菁锌光动力作用的影响。

E Krajewska, M Bryszewska, I V Chapman
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引用次数: 2

摘要

目的:研究CHO K1细胞内源性谷胱甘肽缺失对酞菁锌(ZnPc)光动力作用的影响。材料与方法:使用HeNe激光器632.5 nm,最大功率输出3.5 mW, Toshiba半导体激光器670 nm,最大功率7 mW。将中国仓鼠卵巢细胞(CHO K1)暴露于光下,2-10 J.利用γ -谷氨酰半胱氨酸合成酶抑制剂——丁硫氨酸亚砜胺,在ZnPc和激光照射前降低细胞还原型谷胱甘肽水平[GSH]。通过用氮净化细胞培养物后细胞氧含量降低80%,研究了细胞内缺氧条件的影响。结果:在通风良好的细胞中,ZnPc的光动力作用使加倍次数减少了29 +/- 6%,图2 (p = 0.01)。降低[GSH]的细胞则没有这种效果(p = 0.1)。当缺氧细胞在正常[GSH]下进行研究时,未观察到光动力效应(p = 0.1)。当使用670 nm激光研究细胞活力时,可以观察到光动力学效应(80%比对照下降,p < 0.001),而不考虑单剂量6 J的细胞[GSH]水平。这种效应在[GSH]正常的细胞中观察到,不同剂量的2 J和更高(63%在2 J时下降,p < 0.001)。结论:以细胞加倍次数为终点,降低[GSH]可抑制ZnPc的光动力学效应。ZnPc的光刺激作用同样受到缺氧条件的抑制。当细胞活力为终点时,无论内源性[GSH]值如何,都可以观察到ZnPc的光动力效应。
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The influence of depleted glutathione levels on the photodynamic action of zinc phthalocyanine in CHO K1 cells.

Objective: The current study focuses on any influence that depletion of endogenous glutathione in CHO K1 cells may have on the photodynamic action of zinc phthalocyanine (ZnPc).

Materials and methods: Two lasers--a HeNe laser, 632.5 nm, maximum power output 3.5 mW, and a Toshiba semiconducting laser, 670 nm, maximum power of 7 mW--were used. Chinese Hamster Ovary cells (CHO K1) were exposed to light, 2-10 J. Cellular reduced glutathione levels [GSH] were depressed prior to exposure to ZnPc and laser light, using buthionine sulphoximine, a potent inhibitor of gamma-glutamylcysteine synthetase. The influence of hypoxic intracellular conditions was studied by reduction of oxygen content of cells by 80% following purging of cell cultures with nitrogen.

Results: In well-aerated cells, doubling times are reduced by the photodynamic action of ZnPc by 29 +/- 6%, fig 2 (p = 0.01). Cells with lowered [GSH] do not show this effect (p = 0.1). When hypoxic cells are studied at normal [GSH], no photodynamic effect is observed (p = 0.1). When cell viability is studied, using the 670-nm laser, a photodynamic effect is observed, (80% fall from controls, p < 0.001), irrespective of the cellular [GSH] level for a single dose of 6 J. This effect is observed in cells with normal [GSH], for varied doses of 2 J and higher (63% fall at 2 J, p < 0.001).

Conclusions: Lowered [GSH] was observed to depress the photodynamic effect of ZnPc when cell-doubling times were the endpoint. The photostimulating effect of ZnPc was similarly suppressed by hypoxic conditions. When cell viability was the endpoint, then a photodynamic effect of ZnPc was observed irrespective of the endogenous [GSH] values.

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