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卟啉和辐射对表皮细胞中铁螯合酶和5-氨基乙酰丙酸合酶的影响。

The effect of porphyrin and radiation on ferrochelatase and 5-aminolevulinic acid synthase in epidermal cells.

作者信息

He D, Behar S, Nomura N, Sassa S, Taketani S, Lim H W

机构信息

Dermatology Service, Department of Veterans Affairs Medical Center, NY 10010, USA.

出版信息

Photodermatol Photoimmunol Photomed. 1995 Feb;11(1):25-30. doi: 10.1111/j.1600-0781.1995.tb00134.x.

DOI:10.1111/j.1600-0781.1995.tb00134.x
PMID:7654564
Abstract

The effects of ultraviolet A (UVA) and blue light on ferrochelatase protein, and its mRNA level, in 5-aminolevulinic acid (ALA)-loaded A431 cells was evaluated. Western blot analysis of ferrochelatase protein showed a protein band of 43 kDa. There was a decrease in the protein concentration 24 h and 48 h after irradiation of these cells. In contrast, as judged by Northern blot analysis, there was no change in ferrochelatase mRNA level. Measurement of ALA synthase activity showed an ALA dose-dependent but radiation-independent decrease of enzyme activity, suggesting an end-product feedback inhibition. Since reactive oxygen species generated by porphyrin-induced photochemical reaction may be involved in the decrease in ferrochelatase protein, the effect of scavengers of reactive oxygen species was evaluated by measuring porphyrin accumulation in irradiated, ALA-loaded A431 cells. Porphyrin accumulation was significantly decreased in the presence of singlet oxygen scavenger sodium azide (0.05 mM, 40.6% suppression) or hydroxyl radical scavenger mannitol (5.0 mM, 45.0% suppression). These data suggest that the photochemical reaction induced by porphyrin and irradiation resulted in a decrease in ferrochelatase protein content, but had no effect on ferrochelatase mRNA level nor on ALA synthase activity. The decrease in protein was partly mediated by the reactive oxygen species.

摘要

评估了紫外线A(UVA)和蓝光对5-氨基酮戊酸(ALA)负载的A431细胞中铁螯合酶蛋白及其mRNA水平的影响。铁螯合酶蛋白的蛋白质印迹分析显示有一条43 kDa的蛋白条带。这些细胞照射后24小时和48小时蛋白质浓度降低。相比之下,通过Northern印迹分析判断,铁螯合酶mRNA水平没有变化。ALA合酶活性的测量显示酶活性呈ALA剂量依赖性但与辐射无关的降低,提示存在终产物反馈抑制。由于卟啉诱导的光化学反应产生的活性氧可能参与了铁螯合酶蛋白的减少,因此通过测量照射的、ALA负载的A431细胞中的卟啉积累来评估活性氧清除剂的作用。在单线态氧清除剂叠氮化钠(0.05 mM,抑制40.6%)或羟基自由基清除剂甘露醇(5.0 mM,抑制45.0%)存在的情况下,卟啉积累显著降低。这些数据表明,卟啉和照射诱导的光化学反应导致铁螯合酶蛋白含量降低,但对铁螯合酶mRNA水平和ALA合酶活性没有影响。蛋白质的减少部分由活性氧介导。

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