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Zinc induces caspase-dependent mitochondrial pathway of the programmed cell death in haemocytes of Drosophila melanogaster

机译:锌诱导果蝇血细胞中程序性细胞死亡的半胱天冬酶依赖性线粒体途径

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摘要

Zinc is an essential trace element in cells. However, its high level in cytoplasm promotes activation of stress signaling pathways and may lead to cell death. In the present study we used Drosophila melanogaster blood cells (haemocytes), obtained from the third instar larvae, to study the effects of high concentrations of Zn2+ on programmed cell death (PCD). We analyzed the activity of caspases, the level of caspase inhibitor protein DIAP1 and metallothioneins, as well as calcium concentrations and activity of mitochondria in haemocytes exposed to 0.35 and 1.7 mM concentrations of Zn. The obtained results showed that rapid increase of [Zn2+]i in the cytoplasm up-regulates metallothionein MtnB but not MtnA gene expression in cells treated with Zn2+ in both concentrations. Excess of Zn2+ also induced activation of the initiator caspase Dronc, associated with the mitochondrial pathway of PCD, and the effector caspase DrICE. In turn, the activity of receptor-regulated Dredd caspase was not changed. The level of DIAP1 decreased significantly in haemocytes in the presence of high Zn2+ concentration in comparison to untreated cells. Moreover, mitochondrial membrane potential was significantly decreased after exposure to Zn ions. These results indicate that high concentration of Zn2+ in the cytoplasm of haemocytes induces PCD via a mitochondrial pathway and that caspases play a pivotal role in this process.
机译:锌是细胞中必需的微量元素。然而,其在细胞质中的高水平促进了应激信号通路的活化,并可能导致细胞死亡。在本研究中,我们使用从第三龄幼虫幼虫获得的果蝇果蝇血细胞(血细胞)来研究高浓度的Zn 2 + 对程序性细胞死亡(PCD)的影响。我们分析了胱天蛋白酶的活性,胱天蛋白酶抑制剂蛋白DIAP1和金属硫蛋白的水平,以及暴露于0.35和1.7mM锌浓度的血细胞中钙的浓度和线粒体的活性。获得的结果表明,在细胞质中[Zn 2 + ] i的快速增加均上调了金属硫蛋白MtnB的表达,但没有升高MtnA基因的表达。浓度。过量的Zn 2 + 也会诱导启动子半胱天冬酶Dronc的活化,与PCD的线粒体途径有关,以及效应子半胱天冬酶DrICE。反过来,受体调节的Dredd caspase的活性没有改变。与未处理的细胞相比,在高Zn 2 + 浓度的存在下,血细胞中DIAP1的水平显着降低。此外,暴露于锌离子后,线粒体膜电位显着降低。这些结果表明在血细胞的细胞质中高浓度的Zn 2 + 通过线粒体途径诱导PCD,而胱天蛋白酶在这一过程中起着关键作用。

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