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本文引用的文献

1
Dissection of TMEM165 function in Golgi glycosylation and its Mn sensitivity.TMEM165 功能在高尔基体糖基化及其对锰敏感性中的作用解析。
Biochimie. 2019 Oct;165:123-130. doi: 10.1016/j.biochi.2019.07.016. Epub 2019 Jul 24.
2
Chloroplast-localized BICAT proteins shape stromal calcium signals and are required for efficient photosynthesis.定位于叶绿体的 BICAT 蛋白塑造基质钙信号,并对高效光合作用是必需的。
New Phytol. 2019 Jan;221(2):866-880. doi: 10.1111/nph.15407. Epub 2018 Aug 31.
3
The yeast protein Gdt1p transports Mn ions and thereby regulates manganese homeostasis in the Golgi.酵母蛋白 Gdt1p 转运 Mn 离子,从而调节高尔基体中的锰稳态。
J Biol Chem. 2018 May 25;293(21):8048-8055. doi: 10.1074/jbc.RA118.002324. Epub 2018 Apr 9.
4
Investigating the function of Gdt1p in yeast Golgi glycosylation.研究 Gdt1p 在酵母高尔基体糖基化中的功能。
Biochim Biophys Acta Gen Subj. 2018 Mar;1862(3):394-402. doi: 10.1016/j.bbagen.2017.11.006. Epub 2017 Nov 3.
5
Manganese-induced turnover of TMEM165.锰诱导的跨膜蛋白165(TMEM165)周转
Biochem J. 2017 Apr 19;474(9):1481-1493. doi: 10.1042/BCJ20160910.
6
Acidic and uncharged polar residues in the consensus motifs of the yeast Ca transporter Gdt1p are required for calcium transport.酵母钙转运蛋白Gdt1p共有基序中的酸性和不带电荷的极性残基是钙转运所必需的。
Cell Microbiol. 2017 Jul;19(7). doi: 10.1111/cmi.12729. Epub 2017 Feb 15.
7
Yeast Gdt1 is a Golgi-localized calcium transporter required for stress-induced calcium signaling and protein glycosylation.酵母 Gdt1 是一种定位于高尔基体的钙转运蛋白,对于应激诱导的钙信号和蛋白质糖基化是必需的。
Sci Rep. 2016 Apr 14;6:24282. doi: 10.1038/srep24282.
8
The Evolutionarily Conserved Protein PHOTOSYNTHESIS AFFECTED MUTANT71 Is Required for Efficient Manganese Uptake at the Thylakoid Membrane in Arabidopsis.进化保守蛋白光合作用受影响突变体71是拟南芥类囊体膜高效吸收锰所必需的。
Plant Cell. 2016 Apr;28(4):892-910. doi: 10.1105/tpc.15.00812. Epub 2016 Mar 28.
9
Glycosylation abnormalities in Gdt1p/TMEM165 deficient cells result from a defect in Golgi manganese homeostasis.Gdt1p/TMEM165缺陷细胞中的糖基化异常是由高尔基体锰稳态缺陷引起的。
Hum Mol Genet. 2016 Apr 15;25(8):1489-500. doi: 10.1093/hmg/ddw026. Epub 2016 Feb 1.
10
SLC39A8 Deficiency: A Disorder of Manganese Transport and Glycosylation.溶质载体家族39成员8缺乏症:一种锰转运和糖基化紊乱疾病。
Am J Hum Genet. 2015 Dec 3;97(6):894-903. doi: 10.1016/j.ajhg.2015.11.003.

人类高尔基蛋白 TMEM165 在酵母和细菌细胞中运输钙和锰。

The human Golgi protein TMEM165 transports calcium and manganese in yeast and bacterial cells.

机构信息

Louvain Institute of Biomolecular Science and Technology, Université Catholique de Louvain, B-1348 Louvain-la-Neuve, Belgium.

Cellular and Molecular Microbiology Lab, Université Libre de Bruxelles, B-6041 Gosselies, Belgium.

出版信息

J Biol Chem. 2020 Mar 20;295(12):3865-3874. doi: 10.1074/jbc.RA119.012249. Epub 2020 Feb 11.

DOI:10.1074/jbc.RA119.012249
PMID:32047108
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7086029/
Abstract

Cases of congenital disorders of glycosylation (CDG) have been associated with specific mutations within the gene encoding the human Golgi TMEM165 (transmembrane protein 165), belonging to UPF0016 (uncharacterized protein family 0016), a family of secondary ion transporters. To date, members of this family have been reported to be involved in calcium, manganese, and pH homeostases. Although it has been suggested that TMEM165 has cation transport activity, direct evidence for its Ca- and Mn-transporting activities is still lacking. Here, we functionally characterized human TMEM165 by heterologously expressing it in budding yeast () and in the bacterium Protein production in these two microbial hosts was enhanced by codon optimization and truncation of the putatively autoregulatory N terminus of TMEM165. We show that TMEM165 expression in a yeast strain devoid of Golgi Ca and Mn transporters abrogates Ca- and Mn-induced growth defects, excessive Mn accumulation in the cell, and glycosylation defects. Using bacterial cells loaded with the fluorescent Fura-2 probe, we further obtained direct biochemical evidence that TMEM165 mediates Ca and Mn influxes. We also used the yeast and bacterial systems to evaluate the impact of four disease-causing missense mutations identified in individuals with TMEM165-associated CDG. We found that a mutation leading to a E108G substitution within the conserved UPF0016 family motif significantly reduces TMEM165 activity. These results indicate that TMEM165 can transport Ca and Mn, which are both required for proper protein glycosylation in cells. Our work also provides tools to better understand the pathogenicity of CDG-associated mutations.

摘要

已经有病例将先天性糖基化障碍(CDG)与编码人类高尔基体 TMEM165(跨膜蛋白 165)的基因中的特定突变联系起来,该基因属于 UPF0016(未鉴定的蛋白质家族 0016),这是一个二次离子转运蛋白家族。迄今为止,已有报道称该家族的成员参与钙、锰和 pH 稳态的调节。虽然已经有人提出 TMEM165 具有阳离子转运活性,但缺乏直接证据证明其具有 Ca 和 Mn 转运活性。在这里,我们通过在芽殖酵母()和细菌中异源表达 TMEM165 来对其进行功能表征。在这两种微生物宿主中,通过密码子优化和截短 TMEM165 的推定自身调节 N 端,提高了蛋白的生产。我们表明,在缺乏高尔基体 Ca 和 Mn 转运体的酵母菌株中表达 TMEM165 可以消除 Ca 和 Mn 诱导的生长缺陷、细胞内过量的 Mn 积累以及糖基化缺陷。使用用荧光 Fura-2 探针负载的细菌细胞,我们进一步获得了直接的生化证据,证明 TMEM165 介导 Ca 和 Mn 的内流。我们还使用酵母和细菌系统来评估在 TMEM165 相关 CDG 个体中发现的四个致病错义突变的影响。我们发现,导致保守的 UPF0016 家族基序内 E108G 取代的突变显著降低了 TMEM165 的活性。这些结果表明,TMEM165 可以转运 Ca 和 Mn,这两者都是细胞中正确蛋白质糖基化所必需的。我们的工作还提供了工具来更好地理解与 CDG 相关的突变的致病性。