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

被引:34
作者
Stribny, Jiri [1 ]
Thines, Louise [1 ]
Deschamps, Antoine [1 ]
Goffin, Philippe [2 ]
Morsomme, Pierre [1 ]
机构
[1] Catholic Univ Louvain, Louvain Inst Biomol Sci & Technol, B-1348 Louvain La Neuve, Belgium
[2] Univ Libre Bruxelles, Cellular & Mol Microbiol Lab, B-6041 Gosselies, Belgium
关键词
membrane transport; calcium transport; manganese; Golgi; glycosylation; yeast; CDG; TMEM165; LACTOCOCCUS-LACTIS; DEFICIENCY; TRANSFORMATION; GLYCOSYLATION; MUTATIONS; MEMBRANE; DISORDER;
D O I
10.1074/jbc.RA119.012249
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
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 Ca2+- and Mn2+-transporting activities is still lacking. Here, we functionally characterized human TMEM165 by heterologously expressing it in budding yeast (Saccharomyces cerevisiae) and in the bacterium Lactococcus lactis. 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 Ca2+ and Mn2+ transporters abrogates Ca2+- and Mn2+-induced growth defects, excessive Mn2+ 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 Ca2+ and Mn2+ 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 Ca2+ and Mn2+, which are both required for proper protein glycosylation in cells. Our work also provides tools to better understand the pathogenicity of CDG-associated TMEM165 mutations.
引用
收藏
页码:3865 / 3874
页数:10
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