4.7 Article

Isolation and Quantification of MicroRNAs from Urinary Exosomes/Microvesicles for Biomarker Discovery

Journal

INTERNATIONAL JOURNAL OF BIOLOGICAL SCIENCES
Volume 9, Issue 10, Pages 1021-1031

Publisher

IVYSPRING INT PUBL
DOI: 10.7150/ijbs.6100

Keywords

chronic kidney disease; exosome; miRNA; urine; biomarker

Funding

  1. National Natural Science Foundation of China [81100544, 81130010]
  2. Natural Science Foundation of Jiangsu Province [BK2011602, BK2011061]
  3. major State Basic Research Development Program [2012CB517706]
  4. Research Fund for the Doctoral Program of Ministry of Education [20110092120059]

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Recent studies indicate that microRNA (miRNA) is contained within exosome. Here we sought to optimize the methodologies for the isolation and quantification of urinary exosomal microRNA as a prelude to biomarker discovery studies. Exosomes were isolated through ultracentrifugation and characterized by immunoelectron microscopy. To determine the RNA was confined inside exosomes, the pellet was treated with RNase before RNA isolation. The minimum urine volume, storage conditions for exosomes and exosomal miRNA was evaluated. The presence of miRNAs in patients with various kidney diseases was validated with real-time PCR. The result shows that miRNAs extracted from the exosomal fraction were resistant to RNase digestion and with high quality confirmed by agarose electrophoresis. 16ml of urine was sufficient for miRNA isolation by absolute quantification with 4.15x10(5) copies/ul for miR-200c. Exosomes was stable at 4 degrees C 24h for shipping before stored at -80 degrees C and was stable in urine when stored at -80 degrees C for 12months. Exosomal miRNA was detectable despite 5 repeat freeze-thaw cycles. The detection of miRNA by quantitative PCR showed high reproducibility (>94% for intra-assay and >76% for inter-assay), high sensitivity (positive call 100% for CKD patients), broad dynamic range (8-log wide) and good linearity for quantification (R-2>0.99). miR-29c and miR-200c showed different expression in different types of kidney disease. In summary, the presence of urinary exosomal miRNA was confirmed for patients with a diversity of chronic kidney disease. The conditions of urine collection, storage and miRNA detection determined in this study may be useful for future biomarker discovery efforts.

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