Surface Glycosylation Profiles of Urine Extracellular Vesicles

Gerlach, Jared Q.; Krüger, Anja; Gallogly, S.; Hanley, Seán; Hogan, Marie C.; Ward, Christopher J.; Joshi, Lokesh; Griffin, Matthew D.

doi:10.1371/journal.pone.0074801

Cited by 101 publications

(109 citation statements)

References 59 publications

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“…However, glycosylation of exosomal proteins is widely unknown with the exception of classes of glycans on the surface as evidenced by lectin binding assays. This surface glycome is known to change in autosomal dominant polycystic kidney disease compared with healthy volunteers' urinary exosomes (30). In this study, we have characterized multiple glycoproteins, their N-glycosylation site, glycan compositions, and structures.…”

Section: Resultsmentioning

confidence: 99%

N-linked (N-) Glycoproteomics of Urimary Exosomes*

Saraswat

Joenväära

Musante

et al. 2015

Molecular & Cellular Proteomics

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Epithelial cells lining the urinary tract secrete urinary exosomes (40 -100 nm) that can be targeted to specific cells modulating their functionality. One potential targeting mechanism is adhesion between vesicle surface glycoproteins and target cells. This makes the glycopeptide analysis of exosomes important. Exosomes reflect the physiological state of the parent cells; therefore, they are a good source of biomarkers for urological and other diseases. Moreover, the urine collection is easy and noninvasive and urinary exosomes give information about renal and systemic organ systems. Accordingly, multiple studies on proteomic characterization of urinary exosomes in health and disease have been published. However, no systematic analysis of their glycoproteomic profile has been carried out to date, whereas a conserved glycan signature has been found for exosomes from urine and other sources including T cell lines and human milk.Here, we have enriched and identified the N-glycopeptides from these vesicles. These enriched N-glycopeptides were solved for their peptide sequence, glycan composition, structure, and glycosylation site using collision-induced dissociation MS/MS (CID-tandem MS) data interpreted by a publicly available software GlycopeptideId. Released glycans from the same sample was also analyzed with MALDI-MS.We have identified the N-glycoproteome of urinary exosomes. In total 126 N-glycopeptides from 51 N-glycosylation sites belonging to 37 glycoproteins were found in our results. The peptide sequences of these N-glycopeptides were identified unambiguously and their glycan composition (for 125 N-glycopeptides) and structures (for 87 Nglycopeptides) were proposed. A corresponding glycomic analysis with released N-glycans was also performed. We identified 66 unique nonmodified N-glycan compositions and in addition 13 sulfated/phosphorylated glycans were also found. This is the first systematic analysis of Nglycoproteome of urinary exosomes. Molecular & Cellular Proteomics

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Section: Resultsmentioning

confidence: 99%

N-linked (N-) Glycoproteomics of Urimary Exosomes*

Saraswat

Joenväära

Musante

et al. 2015

Molecular & Cellular Proteomics

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“…90 These proteins and others, such as Cystin and ADP ribosylation factor-like 6, have been found in uEX of patients with PKD. 13,27 Another approach to find a novel diagnostic/monitoring tool for PKD was the study of lectin profiles of uEVs, 91 showing that lectin microarray profiles of uEVs of patients with PKD and healthy controls have different patterns. This suggests possible diseasespecific modifications.…”

Section: Tubular Diseasementioning

confidence: 99%

Extracellular Vesicles in Renal Diseases

Erdbrügger

2016

Journal of the American Society of Nephrology

168

175

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Extracellular vesicles from the urine and circulation have gained significant interest as potential diagnostic biomarkers in renal diseases. Urinary extracellular vesicles contain proteins from all sections of the nephron, whereas most studied circulating extracellular vesicles are derived from platelets, immune cells, and the endothelium. In addition to their diagnostic role as markers of kidney and vascular damage, extracellular vesicles may have functional significance in renal health and disease by facilitating communication between cells and protecting against kidney injury and bacterial infection in the urinary tract. However, the current understanding of extracellular vesicles has derived mostly from studies with very small numbers of patients or in vitro data. Moreover, accurate assessment of these vesicles remains a challenge, in part because of a lack of consensus in the methodologies to measure extracellular vesicles and the inability of most techniques to capture the entire size range of these vesicles. However, newer techniques and standardized protocols to improve the detection of extracellular vesicles are in development. A clearer understanding of the composition and biology of extracellular vesicles will provide insights into their pathophysiologic, diagnostic, and therapeutic roles.

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“…To overcome this problem, THP depolymerization by DTT (dithiothreitol) treatment (18) or uEV isolation by sucrose gradient centrifugation (15,16,19,20) have been routinely used, but both approaches have disadvantages (12,16,21,22). Even when DTT is used, THP can still be present in the isolated uEVs (15,21,23,24), whereas separation on sucrose gradients or cushions (15,19,20) is time-consuming, taking up to 24 hours (15,16,19,20).…”

mentioning

confidence: 99%

Isolation of Urinary Extracellular Vesicles from Tamm- Horsfall Protein–depleted Urine and their Application in the Development of a Lectin-Exosome-Binding Assay

Kosanović

Janković

2014

BioTechniques

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Urine is a readily available source of relatively large quantities of extracellular vesicles (EVs). However, the isolation of urinary EVs (uEVs) is complicated by the presence of Tamm-Horsfall protein (THP), which polymerizes and co-precipitates as a contaminant. This may make glycan analysis of uEVs difficult since THP is heavily glycosylated. To facilitate glycosylation analysis and address the need for elimination of non-uEV glycans, we present a modification of the uEV isolation procedure and use the isolated uEVs in the development of a lectin-exosome binding assay. Salt precipitation was employed to remove THP under conditions originally described for its separation from urine, followed by differential centrifugation. The quality of the isolated uEVs was examined by electron microscopy, SDS-PAGE, and immunoblotting. The uEVs were subsequently immobilized on solid phase and probed with labeled plant lectins using the lectin-exosome binding assay. Our results indicate that the isolated uEVs had preserved structural integrity and reacted with labeled plant lectins in a selective, carbohydrate-dependent manner. The basic lectin binding pattern of uEVs obtained by our method can be used as a reference for assessing the composition of their surface glycans in different physiological and pathological conditions.

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Surface Glycosylation Profiles of Urine Extracellular Vesicles

Cited by 101 publications

References 59 publications

N-linked (N-) Glycoproteomics of Urimary Exosomes*

N-linked (N-) Glycoproteomics of Urimary Exosomes*

Extracellular Vesicles in Renal Diseases

Isolation of Urinary Extracellular Vesicles from Tamm- Horsfall Protein–depleted Urine and their Application in the Development of a Lectin-Exosome-Binding Assay

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