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锌依赖的溶酶体增大在 TRPML1 缺陷细胞中涉及 MTF-1 转录因子和 ZnT4(Slc30a4)转运体。

Zinc-dependent lysosomal enlargement in TRPML1-deficient cells involves MTF-1 transcription factor and ZnT4 (Slc30a4) transporter.

机构信息

Department of Biological Sciences, University of Pittsburgh, Pittsburgh, PA 15260, USA.

出版信息

Biochem J. 2013 Apr 15;451(2):155-63. doi: 10.1042/BJ20121506.

Abstract

Zinc is critical for a multitude of cellular processes, including gene expression, secretion and enzymatic activities. Cellular zinc is controlled by zinc-chelating proteins and by zinc transporters. The recent identification of zinc permeability of the lysosomal ion channel TRPML1 (transient receptor potential mucolipin 1), and the evidence of abnormal zinc levels in cells deficient in TRPML1, suggested a role for TRPML1 in zinc transport. In the present study we provide new evidence for such a role and identify additional cellular components responsible for it. In agreement with the previously published data, an acute siRNA (small interfering RNA)-driven TRPML1 KD (knockdown) leads to the build-up of large cytoplasmic vesicles positive for LysoTracker™ and zinc staining, when cells are exposed to high concentrations of zinc. We now show that lysosomal enlargement and zinc build-up in TRPML1-KD cells exposed to zinc are ameliorated by KD of the zinc-sensitive transcription factor MTF-1 (metal-regulatory-element-binding transcription factor-1) or the zinc transporter ZnT4. TRPML1 KD is associated with a build-up of cytoplasmic zinc and with enhanced transcriptional response of mRNA for MT2a (metallothionein 2a). TRPML1 KD did not suppress lysosomal secretion, but it did delay zinc leak from the lysosomes into the cytoplasm. These results underscore a role for TRPML1 in zinc metabolism. Furthermore, they suggest that TRPML1 works in concert with ZnT4 to regulate zinc translocation between the cytoplasm and lysosomes.

摘要

锌对于许多细胞过程至关重要,包括基因表达、分泌和酶活性。细胞内的锌由锌螯合蛋白和锌转运体控制。最近发现溶酶体离子通道 TRPML1(瞬时受体电位 mucolipin 1)具有锌通透性,并且在 TRPML1 缺陷的细胞中存在异常的锌水平,这表明 TRPML1 在锌转运中起作用。在本研究中,我们提供了新的证据来支持这一作用,并确定了其他负责这一作用的细胞成分。与之前发表的数据一致,急性 siRNA(小干扰 RNA)驱动的 TRPML1 KD(敲低)导致细胞暴露在高浓度锌时,细胞质中出现大的 LysoTracker™和锌染色阳性的囊泡。我们现在表明,TRPML1-KD 细胞暴露于锌时溶酶体增大和锌积累可以通过 KD 锌敏感转录因子 MTF-1(金属调节元件结合转录因子-1)或锌转运体 ZnT4 得到改善。TRPML1 KD 与细胞质中锌的积累以及 MT2a(金属硫蛋白 2a)mRNA 的转录反应增强有关。TRPML1 KD 并没有抑制溶酶体分泌,但它确实延迟了锌从溶酶体漏入细胞质。这些结果强调了 TRPML1 在锌代谢中的作用。此外,它们表明 TRPML1 与 ZnT4 协同作用,调节细胞质和溶酶体之间的锌转运。

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