The Role of N-Glycosylation in Maintaining the Transporter Activity and Expression of Human Oligopeptide Transporter 1

Ting Chan; Xiaoxi Lu; Tahiatul Shams; Ling Zhu; Michael Murray; Fanfan Zhou

doi:10.1021/acs.molpharmaceut.6b00462

The Role of N-Glycosylation in Maintaining the Transporter Activity and Expression of Human Oligopeptide Transporter 1

Mol Pharm. 2016 Oct 3;13(10):3449-3456. doi: 10.1021/acs.molpharmaceut.6b00462. Epub 2016 Sep 2.

Authors

Ting Chan¹, Xiaoxi Lu¹, Tahiatul Shams¹, Ling Zhu², Michael Murray³, Fanfan Zhou¹

Affiliations

¹ Faculty of Pharmacy, The University of Sydney , Sydney, NSW 2006, Australia.
² Retinal Therapeutics Research Group, Save Sight Institute, The University of Sydney , Sydney, NSW 2000, Australia.
³ Pharmacogenomics and Drug Development Group, Discipline of Pharmacology, School of Medical Sciences, The University of Sydney , Sydney, NSW 2006, Australia.

PMID: 27547863
DOI: 10.1021/acs.molpharmaceut.6b00462

Abstract

Human oligopeptide transporter 1 (hPepT1) mediates the absorption of dietary peptides and a range of clinically relevant drugs. According to the predicted topological structure, hPepT1 contains multiple asparagine residues in putative N-glycosylation sites. This study investigated the influence of the six putative N-glycosylation sites within the extracellular region between transmembrane domains 9 and 10 on hPepT1 transporter function and expression in HEK-293T cells. Our study confirmed that hPepT1 is N-glycosylated in HEK-293T cells with the glycosylated and fully deglycosylated isoforms exhibiting apparent molecular masses of ∼78 and ∼55 kDa, respectively. Transport uptake of Glycylsarcosine (Gly-sar) by the hPepT1-N562Q variant, but not by other single mutants, was moderately impaired. We also constructed multiple N-glycosylation mutants based on the hPepT1-N562Q mutant by mutagenizing the additional asparagine residues N404Q, N408Q, N439Q, N509Q, and N514Q. Transport function showed a graded decrease as the number of mutagenized residues increased and simultaneous removal of all six asparagine residues essentially abolished transport activity. Kinetic studies indicated that the V_max values for Gly-sar transport by low activity mutants were decreased compared to those of wild-type, which suggested that the cell surface expression and/or turnover rate of hPepT1 mutants was impaired; K_m values were unchanged in most cases. Using immunoblotting and immunofluorescence, the plasma membrane and total cellular expression of the mutant transporters were decreased in accordance with functional impairments. In summary, we provide the first molecular evidence that hPepT1 is modified by N-glycosylation and that all six asparagine residues in the large extracellular loop between transmembrane domains 9 and 10 are subject to N-glycosylation. This information enhances our understanding of the role of the large extracellular loop in hPepT1 regulation and could facilitate the development of new hPepT1 substrate drugs with improved bioavailability.

Keywords: N-glycosylation; human oligopeptide transporter 1; post-translational modification; transport activity; transporter expression.

MeSH terms

Biological Transport / genetics
Biological Transport / physiology
Biotinylation
Cell Line
Fluorescent Antibody Technique
Glycosylation
Humans
Immunoblotting
Kinetics
Mutagenesis, Site-Directed
Peptide Transporter 1
Protein Isoforms / genetics
Protein Isoforms / metabolism
Protein Processing, Post-Translational
Symporters / genetics
Symporters / metabolism*

Substances

Peptide Transporter 1
Protein Isoforms
SLC15A1 protein, human
Symporters