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The influence of zinc status onp53 tumor suppressor gene expression and p53 target genes in human hepatoblastoma, bronchial epithelial, and aortic endothelial cells

机译:锌状态对人肝母细胞瘤,支气管上皮和主动脉内皮细胞中p53抑癌基因表达和p53靶基因的影响

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摘要

The influence of zinc status on the expression of p53, the human tumor suppressor gene as well as downstream target genes of p53 were examined in human cell lines. HepG2 cells were depleted of cellular zinc using a low-zinc media containing Chelex-100 treated serum. Cellular zinc levels were depleted to 64% of controls (4.0 μM zinc, comparable to normal media). p53 mRNA was increased in the zinc-depleted HepG2s as compared to control, however, p53 protein levels and DNA binding activity were not significantly different among treatment groups. NHBEs were depleted of zinc using a serum-free zinc-free media which contained residual amounts of zinc (0.4 μM, ZD). Other treatments included a control group at 4.0 μM of zinc (ZN), for comparison with normal media, 16.0 μM (ZA), for comparison with human serum levels of zinc, and 32.0 μM (ZS), an attainable level of zinc supplementation in humans. Zinc was reduced to 34% in the ZD group as compared to the ZN control group, however, the ZA group and ZS group were significantly higher than control, 240% and 446% respectively. Using RNase protection assays, p53 and gadd45 mRNA were increased almost 100% in the ZD group, as compared to ZN and was higher in the ZA and ZS groups. c-fos was increased 79% in the ZS group as compared to the control group. p53 protein levels were almost 500% higher in the ZD group, and the ZA and ZS groups were six-fold and 16-fold higher respectively, as compared to the ZN group. HAECs were depleted of zinc using a low-serum zinc-free media that contained residual amounts of zinc (0.8 μM, ZD). Other treatments included a control group at 3.0 μM of zinc (ZN), 16.0 μM (ZA), and 32.0 μM (ZS). p53 protein was increased 100% in both the ZD and ZS groups as compared to control, and almost 200% higher in the ZA group. p21, bax and bcl-2, showed significant increases in mRNA in the ZS group as compared to the ZN control group. Mcl-1 mRNA abundance also showed an increase in the ZS cells as compared to ZN control cells.
机译:在人细胞系中检查了锌状态对p53,人类肿瘤抑制基因以及p53下游靶基因表达的影响。使用含有Chelex-100处理的血清的低锌培养基,可以清除HepG2细胞中的锌。细胞锌水平被消耗至对照组的64%(4.0μM锌,与普通培养基相当)。与对照组相比,缺锌的HepG2中p53 mRNA的表达增加,但是,治疗组之间p53蛋白的水平和DNA结合活性没有显着差异。 NHBE使用不含血清的无锌培养基去除锌,该培养基含有残留量的锌(0.4μM,ZD)。其他治疗方法包括对照组(4.0μM锌(ZN)与正常培养基比较),16.0μM(ZA)(与人血清锌水平比较)和32.0μM(ZS)(锌在人体中可达到的补充水平)人类。与ZN对照组相比,ZD组的锌减少到34%,但是ZA组和ZS组的锌显着高于对照组,分别为240%和446%。使用RNase保护试验,与ZN相比,ZD组的p53和gadd45 mRNA几乎增加了100%,而ZA和ZS组则更高。与对照组相比,ZS组的c-fos增加了79%。与ZN组相比,ZD组的p53蛋白水平高出近500%,ZA和ZS组分别高出6倍和16倍。 HAEC使用含有残留锌量(0.8μM,ZD)的低血清无锌培养基消耗锌。其他治疗包括对照组,分别为3.0μM的锌(ZN),16.0μM(ZA)和32.0μM(ZS)。与对照组相比,ZD和ZS组的p53蛋白均增加了100%,而ZA组则提高了近200%。与ZN对照组相比,p21,bax和bcl-2在ZS组中显示出mRNA的显着增加。与ZN对照细胞相比,Mcl-1 mRNA丰度也显示ZS细胞增加。

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    Fanzo Jessica Christine;

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  • 年度 2000
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