首页> 外文期刊>Journal of cellular biochemistry. >Induction of stress response and differential expression of 70 kDa stress proteins by sodium fluoride in HeLa and rat brain tumor 9L cells.
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Induction of stress response and differential expression of 70 kDa stress proteins by sodium fluoride in HeLa and rat brain tumor 9L cells.

机译:氟化钠在HeLa和大鼠脑肿瘤9L细胞中诱导70kDa应激蛋白的应激响应和差异表达。

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We herein demonstrate that sodium fluoride (NaF) acts as a stress response inducer on HeLa and 9L rat brain tumor cells. NaF is only slightly cytotoxic, and inhibitory to Ser/Thr-phosphatases but not to Tyr-phosphatases in both cell lines. After treatment with 5 mM NaF for 2 h, the phosphorylation levels of vimentin and an alkali-resistant 65-kDa phosphoprotein were enhanced, a common phenomenon detected in cells under a variety of stress conditions. Under an identical treatment protocol, in which the cells were treated with 5 mM NaF for 2 h and then allowed to recover under normal growing conditions for up to 12 h, NaF differentially induced the cytoplasmic/nuclear heat-shock protein70s (including both the inducible and the constitutively expressed members of this protein family) in HeLa cells and the endoplasmic reticulum residing heat-shock protein70 (the glucose-regulated protein with an apparent molecular weight of 78 kDa) in 9L cells. Electrophoretic mobility shift assays (EMSA) using probes containing well-characterized regulatory elements revealed the activation of the heat-shock factor in HeLa but not in 9L cells; this is in good agreement with the stress protein induction pattern. Additional differential induction of binding activities toward EMSA probes individually containing NF-KB, AP-2, and CRE-like elements were detected in NaF-treated cells. The possible involvement of these binding sites as well as the corresponding factors in the stress response are discussed.
机译:我们在本文中表明氟化钠(NAF)在Hela和9L大鼠脑肿瘤细胞上用作应力反应诱导剂。 NAF仅略微细胞毒性,并抑制SER / THR-磷酸酶,但在两种细胞系中没有磷酸酶。在用5mM NAF处理2小时后,增强了Vimentin和耐碱的65-KDA磷蛋白的磷酸化水平,在各种应力​​条件下在细胞中检测到常见现象。在相同的处理方案下,用5mM NAF处理细胞2小时,然后在正常生长条件下恢复至多12小时,NAF差异诱导细胞质/核热休克蛋白质70s(包括诱导型在9L细胞中,在HeLa细胞和内质网的组成蛋白质系列的成员)在HeLa细胞和内质网偏离热休克蛋白质70中,在9L细胞中具有78kda的表观分子量的葡萄糖调节蛋白。使用含有良好表征的调节元件的探针的电泳迁移率移位测定(EMSA)显示Hela中的热休克因子,但不含9L细胞;这与应激蛋白质诱导模式吻合良好。在NAF处理的细胞中检测到单独含有NF-KB,AP-2和CRE样元件对EMSA探针的结合活性的额外差异诱导。讨论了这些结合位点的可能参与以及应力响应中的相应因子。

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