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Detailed N-glycan analysis of mannose receptor purified from murine spleen indicates tissue specific sialylation
Authors:Yunpeng Su  Louise Royle  Catherine M Radcliffe  David J Harvey  Luisa Martinez-Pomares  Pauline M Rudd
Institution:a Glycobiology Institute, Biochemistry Department, University of Oxford, South Parks Road, OX1, 3QU, United Kingdom
b Sir William’s Dunn School of Pathology, University of Oxford, South Parks Road, OX1, 3QU, United Kingdom
Abstract:The mannose receptor (MR) is a heavily glycosylated endocytic receptor that recognises both mannosylated and sulphated ligands through its C-type lectin domains (CTLDs) and cysteine-rich (CR) domain, respectively. It is widely expressed among different tissues and by certain cell types in vivo. Our previous study suggested that the glycosylation, especially terminal sialylation, regulated the functional specificities of MR. In the current investigation, the distribution of MR among various mouse tissues was studied and the N-linked glycosylation of spleen MR was analysed. Our results showed that spleen expressed the most abundant MR, consistent with its wide distribution in different cell types in this organ. Spleen MR was heterogeneously N-glycosylated. The majority of the glycans were sialylated in the α2 → 6-linkage and both Neu5Ac and Neu5Gc sialic acids were detected. Most glycans were bi-antennary (74%) with ∼22% tri-antennary and most were core fucosylated (68%). About 13% contained α-galactose. In the lung, MR exhibited more terminal sialic acids in the α2 → 3- rather than in the α2 → 6-configuration. Our study provides a profile of MR N-linked glycosylation that will facilitate our understanding of their physiological role on MR biology in vivo.
Keywords:2-AB  2-aminobenzamide  CTLDs  C-type lectin domains  CR  cysteine-rich domain  GlcNAc  N-acetylglucosamine  ESI  electrospray ionization  GU  glucose unit  HPLC  high-performance liquid chromatography  IEF  isoelectric focusing  LC/MS  liquid chromatography/mass spectrometry  MALDI  matrix-assisted laser desorption/ionization  MR  mannose receptor  MS  mass spectrometry  MS/MS  tandem mass spectrometry  NP  normal phase  PAGE  polyacrylamide gel electrophoresis  PNGase F  peptide N-glycosidase F  SDS  sodium dodecyl sulfate  TFA  trifluoroacetic acid  TOF  time-of-flight  WAX  weak anion exchange
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