Lectin-induced agglutination method of urinary exosomes isolation followed by mi-RNA analysis: Application for prostate cancer diagnostic

Roman Samsonov; Tatiana Shtam; Vladimir Burdakov; Andrey Glotov; Evgenia Tsyrlina; Lev Berstein; Alexander Nosov; Vladimir Evtushenko; Michael Filatov; Anastasia Malek

doi:10.1002/pros.23101

Lectin-induced agglutination method of urinary exosomes isolation followed by mi-RNA analysis: Application for prostate cancer diagnostic

Prostate. 2016 Jan;76(1):68-79. doi: 10.1002/pros.23101. Epub 2015 Sep 29.

Authors

Affiliations

¹ Laboratory of Oncoendocrinology, N.N. Petrov Institute of Oncology, Pesochny, Saint-Petersburg, Russia.
² Laboratory of Genetic Engineering, Russian Research Centre for Radiology and Surgical Technologies, St. Petersburg, Russia.
³ Division of Molecular and Radiation Biophysics, SFBI Petersburg Nuclear Physics Institute, Gatchina, Saint-Petersburg, Russia.
⁴ Department of Genetics and Biotechnology, Saint Petersburg State University, Saint-Petersburg, Russia.
⁵ Department of Urology, N.N. Petrov Institute of Oncology, Pesochny, Saint-Petersburg, Russia.
⁶ Laboratory of Cell Migration and Invasion, Faculty of Medicine in the Galilee, Bar-Ilan University, Safed, Israel.

PMID: 26417675
DOI: 10.1002/pros.23101

Abstract

Background: Prostate cancer is the most common cancer in men. Prostate-specific antigen has, however, insufficient diagnostic specificity. Novel complementary diagnostic approaches are greatly needed. MiRNAs are small regulatory RNAs which play an important role in tumorogenesis and are being investigated as a cancer biomarker. In addition to their intracellular regulatory functions, miRNAs are secreted into the extracellular space and can be found in various body fluids, including urine. The stability of extracellular miRNAs is defined by association with proteins, lipoprotein particles, and membrane vesicles. Among the known forms of miRNA packaging, tumour-derived exosome-enclosed miRNAs is thought to reflect the vital activity of cancer cells. The assessment of the exosomal fraction of urinary miRNA may present a new and highly specific method for prostate cancer diagnostics; however, this is challenged by the absence of reliable and inexpensive methods for isolation of exosomes.

Methods: Prostate cancer (PC) cell lines and urine samples collected from 35 PC patients and 35 healthy donors were used in the study. Lectins, phytohemagglutinin, and concanavalin A were used to induce agglutination of exosomes. The efficiency of isolation process was evaluated by AFM and DLS assays. The protein content of isolated exosomes was analysed by western blotting. Exosomal RNA was assayed by automated electrophoresis and expression level of selected miRNAs was evaluated by RT-qPCR. The diagnostic potency of the urinary exosomal miRNA assessment was estimated by the ROC method.

Results: The formation of multi-vesicular agglutinates in urine can be induced by incubation with lectin at a final concentration of 2 mg/ml. These agglutinates contain urinary exosomes and may be pelleted by centrifugation with a relatively low G-force. The analysis of PC-related miRNA in urinary exosomes revealed significant up-regulation of miR-574-3p, miR-141-5p, and miR-21-5p associated with PC.

Conclusions: Lectin-induced aggregation is a low-cost and easily performed method for isolation of exosomes from urine. Isolated exosomes can be further analysed in terms of miRNA content. The miRNA profile of urinary exosomes reflects development of prostate cancer and may present a promising diagnostic tool.

Keywords: diagnostic; exosomes; lectin; miRNA; prostate cancer.

Publication types

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

MeSH terms

Adult
Aged
Agglutination Tests / methods
Biomarkers / urine
Exosomes / metabolism*
Humans
Lectins / pharmacology
Male
MicroRNAs / urine*
Middle Aged
Neoplasm Grading
Neoplasm Staging
Prostatic Neoplasms* / diagnosis
Prostatic Neoplasms* / pathology
Prostatic Neoplasms* / urine
Reproducibility of Results
Tumor Cells, Cultured

Substances

Biomarkers
Lectins
MicroRNAs