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本文引用的文献

1
TPC2 mediates new mechanisms of platelet dense granule membrane dynamics through regulation of Ca2+ release.TPC2通过调节钙离子释放介导血小板致密颗粒膜动力学的新机制。
Mol Biol Cell. 2015 Sep 15;26(18):3263-74. doi: 10.1091/mbc.E15-01-0058. Epub 2015 Jul 22.
2
Membrane-Associated Transporter Protein (MATP) Regulates Melanosomal pH and Influences Tyrosinase Activity.膜相关转运蛋白(MATP)调节黑素小体pH值并影响酪氨酸酶活性。
PLoS One. 2015 Jun 9;10(6):e0129273. doi: 10.1371/journal.pone.0129273. eCollection 2015.
3
Ebola virus. Two-pore channels control Ebola virus host cell entry and are drug targets for disease treatment.埃博拉病毒。双孔通道控制埃博拉病毒进入宿主细胞,是疾病治疗的药物靶点。
Science. 2015 Feb 27;347(6225):995-8. doi: 10.1126/science.1258758.
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Lysosomal calcium signalling regulates autophagy through calcineurin and ​TFEB.溶酶体钙信号通过钙调神经磷酸酶和 TFEB 调节自噬。
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An intracellular anion channel critical for pigmentation.一种对色素沉着至关重要的细胞内阴离子通道。
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Myosin vc interacts with Rab32 and Rab38 proteins and works in the biogenesis and secretion of melanosomes.肌球蛋白vc与Rab32和Rab38蛋白相互作用,并在黑素小体的生物发生和分泌过程中发挥作用。
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The Two-pore channel (TPC) interactome unmasks isoform-specific roles for TPCs in endolysosomal morphology and cell pigmentation.双孔通道(TPC)相互作用组揭示了TPC在溶酶体形态和细胞色素沉着中的亚型特异性作用。
Proc Natl Acad Sci U S A. 2014 Sep 9;111(36):13087-92. doi: 10.1073/pnas.1407004111. Epub 2014 Aug 25.
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High susceptibility to fatty liver disease in two-pore channel 2-deficient mice.两孔通道 2 缺陷小鼠对脂肪肝疾病的高易感性。
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Genome engineering using the CRISPR-Cas9 system.使用 CRISPR-Cas9 系统进行基因组工程。
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TPC2通过调节黑素小体的pH值和大小来控制色素沉着。

TPC2 controls pigmentation by regulating melanosome pH and size.

作者信息

Ambrosio Andrea L, Boyle Judith A, Aradi Al E, Christian Keith A, Di Pietro Santiago M

机构信息

Department of Biochemistry and Molecular Biology, Colorado State University, Fort Collins, CO 80523-1870.

Department of Biochemistry and Molecular Biology, Colorado State University, Fort Collins, CO 80523-1870

出版信息

Proc Natl Acad Sci U S A. 2016 May 17;113(20):5622-7. doi: 10.1073/pnas.1600108113. Epub 2016 May 2.

DOI:10.1073/pnas.1600108113
PMID:27140606
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4878521/
Abstract

Melanin is responsible for pigmentation of skin and hair and is synthesized in a specialized organelle, the melanosome, in melanocytes. A genome-wide association study revealed that the two pore segment channel 2 (TPCN2) gene is strongly linked to pigmentation variations. TPCN2 encodes the two-pore channel 2 (TPC2) protein, a cation channel. Nevertheless, how TPC2 regulates pigmentation remains unknown. Here, we show that TPC2 is expressed in melanocytes and localizes to the melanosome-limiting membrane and, to a lesser extent, to endolysosomal compartments by confocal fluorescence and immunogold electron microscopy. Immunomagnetic isolation of TPC2-containing organelles confirmed its coresidence with melanosomal markers. TPCN2 knockout by means of clustered regularly interspaced short palindromic repeat/CRISPR-associated 9 gene editing elicited a dramatic increase in pigment content in MNT-1 melanocytic cells. This effect was rescued by transient expression of TPC2-GFP. Consistently, siRNA-mediated knockdown of TPC2 also caused a substantial increase in melanin content in both MNT-1 cells and primary human melanocytes. Using a newly developed genetically encoded pH sensor targeted to melanosomes, we determined that the melanosome lumen in TPC2-KO MNT-1 cells and primary melanocytes subjected to TPC2 knockdown is less acidic than in control cells. Fluorescence and electron microscopy analysis revealed that TPC2-KO MNT-1 cells have significantly larger melanosomes than control cells, but the number of organelles is unchanged. TPC2 likely regulates melanosomes pH and size by mediating Ca(2+) release from the organelle, which is decreased in TPC2-KO MNT-1 cells, as determined with the Ca(2+) sensor tyrosinase-GCaMP6. Thus, our data show that TPC2 regulates pigmentation through two fundamental determinants of melanosome function: pH and size.

摘要

黑色素负责皮肤和毛发的色素沉着,在黑素细胞的一种特殊细胞器黑素小体中合成。一项全基因组关联研究表明,双孔段通道2(TPCN2)基因与色素沉着变异密切相关。TPCN2编码双孔通道2(TPC2)蛋白,一种阳离子通道。然而,TPC2如何调节色素沉着仍不清楚。在这里,我们通过共聚焦荧光和免疫金电子显微镜显示,TPC2在黑素细胞中表达,并定位于黑素小体限制膜,在较小程度上定位于内溶酶体区室。对含TPC2细胞器的免疫磁分离证实了它与黑素小体标记物的共定位。通过成簇规律间隔短回文重复序列/CRISPR相关蛋白9基因编辑敲除TPCN2,导致MNT-1黑素细胞中色素含量显著增加。TPC2-GFP的瞬时表达挽救了这一效应。同样,siRNA介导的TPC2敲低也导致MNT-1细胞和原代人黑素细胞中黑色素含量大幅增加。使用一种新开发的靶向黑素小体的基因编码pH传感器,我们确定TPC2基因敲除的MNT-1细胞和TPC2敲低的原代黑素细胞中的黑素小体腔的酸性低于对照细胞。荧光和电子显微镜分析显示,TPC2基因敲除的MNT-1细胞的黑素小体明显大于对照细胞,但细胞器数量不变。TPC2可能通过介导细胞器中Ca(2+)的释放来调节黑素小体的pH值和大小,如用Ca(2+)传感器酪氨酸酶-GCaMP6所测定的,在TPC2基因敲除的MNT-1细胞中Ca(2+)的释放减少。因此,我们的数据表明,TPC2通过黑素小体功能的两个基本决定因素:pH值和大小来调节色素沉着。