Microarray-based identification of lectins for the purification of human urinary extracellular vesicles directly from urine samples

Juan Echevarria; Felix Royo; Raquel Pazos; Lorena Salazar; Juan Manuel Falcon-Perez; Niels-Christian Reichardt

doi:10.1002/cbic.201402058

Microarray-based identification of lectins for the purification of human urinary extracellular vesicles directly from urine samples

Chembiochem. 2014 Jul 21;15(11):1621-6. doi: 10.1002/cbic.201402058. Epub 2014 Jul 8.

Authors

Juan Echevarria¹, Felix Royo, Raquel Pazos, Lorena Salazar, Juan Manuel Falcon-Perez, Niels-Christian Reichardt

Affiliation

¹ Glycotechnology Laboratory, CIC BiomaGUNE, Paseo Miramon 182, 20009 San Sebastian (Spain).

PMID: 25044519
DOI: 10.1002/cbic.201402058

Abstract

As cellular-derived vesicles largely maintain the biomolecule composition of their original tissue, exosomes, which are found in nearly all body fluids, have enormous potential as clinical disease markers. A major bottleneck in the development of exosome-based diagnostic assays is the challenging purification of these vesicles; this requires time-consuming and instrument-based procedures. We employed lectin arrays to identify potential lectins as probes for affinity-based isolation of exosomes from the urinary matrix. We found three lectins that showed specific interactions to vesicles and no (or only residual) interaction with matrix proteins. Based on these findings a bead-based method for lectin-based isolation of exosomes from urine was developed as a sample preparation step for exosome-based biomarker research.

Keywords: biomarkers; exosomes; glycosylation; microarrays; urine.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Exosomes / chemistry
Exosomes / metabolism*
Humans
Lectins / analysis*
Lectins / isolation & purification
Molecular Probes / analysis*
Molecular Probes / isolation & purification
Protein Array Analysis*
Urine / cytology*

Substances

Lectins
Molecular Probes