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Rft1 catalyzes lipid-linked oligosaccharide translocation across the ER membrane.

Shuai ChenCai-Xia PeiSi XuHanjie LiYi-Shi LiuYicheng WangCheng JinNeta DeanXiao-Dong Gao
Published in: Nature communications (2024)
The eukaryotic asparagine (N)-linked glycan is pre-assembled as a fourteen-sugar oligosaccharide on a lipid carrier in the endoplasmic reticulum (ER). Seven sugars are first added to dolichol pyrophosphate (PP-Dol) on the cytoplasmic face of the ER, generating Man5GlcNAc2-PP-Dol (M5GN2-PP-Dol). M5GN2-PP-Dol is then flipped across the bilayer into the lumen by an ER translocator. Genetic studies identified Rft1 as the M5GN2-PP-Dol flippase in vivo but are at odds with biochemical data suggesting Rft1 is dispensable for flipping in vitro. Thus, the question of whether Rft1 plays a direct or an indirect role during M5GN2-PP-Dol translocation has been controversial for over two decades. We describe a completely reconstituted in vitro assay for M5GN2-PP-Dol translocation and demonstrate that purified Rft1 catalyzes the translocation of M5GN2-PP-Dol across the lipid bilayer. These data, combined with in vitro results demonstrating substrate selectivity and rft1∆ phenotypes, confirm the molecular identity of Rft1 as the M5GN2-PP-Dol ER flippase.
Keyphrases
  • endoplasmic reticulum
  • estrogen receptor
  • breast cancer cells
  • electronic health record
  • fatty acid
  • gene expression
  • dna methylation
  • high throughput
  • genome wide
  • amino acid
  • cell surface