Posttranscriptional Regulation Controls Calretinin Expression in Malignant Pleural Mesothelioma

Jelena Kresoja-Rakic,Steven Kao,Merve Sulemani,Michaela B. Kirschner,Walter Weder,Manuel Ronner,Glen Reid,Emanuela Felley-Bosco,Beat Schwaller,Rolf A. Stahel

doi:10.3389/fgene.2017.00070

Abstract

Calretinin (CALB2) is a diagnostic and prognostic marker in malignant pleural mesothelioma (MPM). We previously reported that calretinin expression is regulated at the mRNA level. The presence of a medium-sized (573 nucleotide) 3′ untranslated region (3′UTR) predicted to contain binding sites for miR-30a/b/c/d/e and miR-9 as well as an adenine/uridine-rich element (ARE) in all three transcripts arising from the CALB2 gene, suggests that calretinin expression is regulated via posttranscriptional mechanisms. Our aim was to investigate the role of the CALB2-3′UTR in the posttranscriptional regulation of calretinin expression in MPM. CALB2-3′UTR was inserted downstream of the luciferase reporter gene using pmiRGLO vector and reporter expression was determined after transfection into MPM cells. Targeted mutagenesis was used to generate variants harboring mutated miR-30 family and ARE binding sites. Electrophoretic mobility shift assay was used to test for the presence of ARE binding proteins. CALB2-3′UTR significantly decreased luciferase activity in MPM cells. Analysis of mutation in the ARE site revealed a further destabilization of the reporter and human antigen R (HuR) binding to the ARE sequence was detected. The mutation of two miR-30 binding sites abolished CALB2-3′UTR destabilization effect; a transient delivery of miR-30e-5p mimics or anti-miR into MPM cells resulted in a significant decrease/increase of the luciferase reporter expression and calretinin protein, respectively. Moreover, overexpression of CALB2-3′UTR quenched the effect of miR-30e-5p mimics on calretinin protein levels, possibly by sequestering the mimics, thereby suggesting a competitive endogenous RNA network. Finally, by data mining we observed that expression of miR-30e-5p was negatively correlated with the calretinin expression in a cohort of MPM patient samples. Our data show the role of (1) adenine-uridine (AU)-binding proteins in calretinin stabilization and (2) miR-30e-5p in the posttranscriptional negative regulation of calretinin expression via interaction with its 3′UTR. Furthermore, our study demonstrates a possible physiological role of calretinin’s alternatively spliced transcripts.

Highlights

Malignant pleural mesothelioma (MPM) is an aggressive form of cancer arising from mesothelial cells lining the pleural cavity and is mainly resulting from the inhalation of asbestos fibers (Porpodis et al, 2013)
In a previous study we demonstrated a strong positive correlation between calretinin mRNA and protein levels in mesothelioma cell lines (Kresoja-Rakic et al, 2016) and demonstrated nuclear respiratory factor 1 (NRF-1) and E2F2 to act as transcription factors regulating calretinin expression
We determined that calretinin expression is regulated in mesothelioma cells through a posttranscriptional mechanism mediated by the 3 untranslated region (3 UTR)

Summary

Introduction

Malignant pleural mesothelioma (MPM) is an aggressive form of cancer arising from mesothelial cells lining the pleural cavity and is mainly resulting from the inhalation of asbestos fibers (Porpodis et al, 2013). Molecular mechanisms driving calretinin expression in mesothelioma remain largely unknown. We have recently described that the expression of calretinin is regulated at the level of transcription by nuclear respiratory factor 1 (NRF-1) and E2F2 transcription factors (Kresoja-Rakic et al, 2016). As the CALB2 mRNA includes a so-called medium size (Fanourgakis et al, 2016) 3 untranslated region (3 UTR) (573 bp) containing an adenine/uridine-rich element (ARE) motif as well as a microRNA (miRNAs) binding sequences, this suggests that posttranscriptional mechanisms of regulation are involved. The ARE motif is the most frequently studied cis-acting element that plays a role in the posttranscriptional control of gene expression by affecting mRNA stability. The most extensively studied AUBPs are HuR/ELAVL1 (human antigen R, embryonic lethal abnormal vision, Drosophila—stabilization; Ma et al, 1996; Brennan and Steitz, 2001), TTP (tristetraprolin), and AUF (ARE/poly(U)binding/degradation factor 1—destabilization) (Barreau et al, 2005)

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