New miRNA profiles accurately distinguish renal cell carcinomas and upper tract urothelial carcinomas from the normal kidney

Apostolos Zaravinos; George I Lambrou; Nikos Mourmouras; Patroklos Katafygiotis; Gregory Papagregoriou; Krinio Giannikou; Dimitris Delakas; Constantinos Deltas

doi:10.1371/journal.pone.0091646

New miRNA profiles accurately distinguish renal cell carcinomas and upper tract urothelial carcinomas from the normal kidney

PLoS One. 2014 Mar 12;9(3):e91646. doi: 10.1371/journal.pone.0091646. eCollection 2014.

Authors

Apostolos Zaravinos¹, George I Lambrou², Nikos Mourmouras³, Patroklos Katafygiotis³, Gregory Papagregoriou⁴, Krinio Giannikou⁵, Dimitris Delakas³, Constantinos Deltas⁴

Affiliations

¹ Molecular Medicine Research Center and Laboratory of Molecular and Medical Genetics, Department of Biological Sciences, University of Cyprus, Nicosia, Cyprus. zaravinos.apostolos@ucy.ac.cy
² Choremeio Research Laboratory, First Department of Pediatrics, University of Athens, Athens, Greece.
³ Department of Urology, Asklipieio General Hospital, Athens, Greece.
⁴ Molecular Medicine Research Center and Laboratory of Molecular and Medical Genetics, Department of Biological Sciences, University of Cyprus, Nicosia, Cyprus.
⁵ Department of Medical Genetics, Medical School, University of Athens, Athens, Greece.

Abstract

Background: Upper tract urothelial carcinomas (UT-UC) can invade the pelvicalyceal system making differential diagnosis of the various histologically distinct renal cell carcinoma (RCC) subtypes and UT-UC, difficult. Correct diagnosis is critical for determining appropriate surgery and post-surgical treatments. We aimed to identify microRNA (miRNA) signatures that can accurately distinguish the most prevalent RCC subtypes and UT-UC form the normal kidney.

Methods and findings: miRNA profiling was performed on FFPE tissue sections from RCC and UT-UC and normal kidney and 434 miRNAs were significantly deregulated in cancerous vs. the normal tissue. Hierarchical clustering distinguished UT-UCs from RCCs and classified the various RCC subtypes among them. qRT-PCR validated the deregulated expression profile for the majority of the miRNAs and ROC analysis revealed their capability to discriminate between tumour and normal kidney. An independent cohort of freshly frozen RCC and UT-UC samples was used to validate the deregulated miRNAs with the best discriminatory ability (AUC>0.8, p<0.001). Many of them were located within cytogenetic regions that were previously reported to be significantly aberrated. miRNA targets were predicted using the miRWalk algorithm and ingenuity pathway analysis identified the canonical pathways and curated networks of the deregulated miRNAs. Using the miRWalk algorithm, we further identified the top anti-correlated mRNA/miRNA pairs, between the deregulated miRNAs from our study and the top co-deregulated mRNAs among 5 independent ccRCC GEO datasets. The AB8/13 undifferentiated podocyte cells were used for functional assays using luciferase reporter constructs and the developmental transcription factor TFCP2L1 was proved to be a true target of miR-489, which was the second most upregulated miRNA in ccRCC.

Conclusions: We identified novel miRNAs specific for each RCC subtype and UT-UC, we investigated their putative targets, the networks and pathways in which they participate and we functionally verified the true targets of the top deregulated miRNAs.

Publication types

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

MeSH terms

Adult
Aged
Aged, 80 and over
Carcinoma, Renal Cell / genetics*
Carcinoma, Renal Cell / pathology
Chromosome Aberrations
Cohort Studies
Female
Gene Expression Profiling
Humans
Kidney / cytology*
Kidney / metabolism
Kidney / pathology*
Kidney Neoplasms / genetics*
Kidney Neoplasms / pathology
Male
MicroRNAs / genetics*
Middle Aged
Urothelium / metabolism*

Substances

MicroRNAs

Grants and funding

This project was funded by the Cyprus Research Promotion Foundation, New Infrastructure/ΣΤΡΑΤΗ/0308/24 (co-funding by the EU Structural Funds) to CD. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.