Promoter methylation inhibits expression of tumor suppressor KIBRA in human clear cell renal cell carcinoma

Katrin Schelleckes; Boris Schmitz; Giuliano Ciarimboli; Malte Lenders; Hermann J. Pavenstädt; Edwin Herrmann; Stefan-Martin Brand; Eva Brand

doi:10.1186/s13148-017-0415-6

Clinical Epigenetics (Oct 2017)

Promoter methylation inhibits expression of tumor suppressor KIBRA in human clear cell renal cell carcinoma

Katrin Schelleckes,
Boris Schmitz,
Giuliano Ciarimboli,
Malte Lenders,
Hermann J. Pavenstädt,
Edwin Herrmann,
Stefan-Martin Brand,
Eva Brand

Affiliations

Katrin Schelleckes: Internal Medicine D, Nephrology, Hypertension and Rheumatology, University Hospital Muenster
Boris Schmitz: Institute of Sports Medicine, Molecular Genetics of Cardiovascular Disease, University Hospital Muenster
Giuliano Ciarimboli: Internal Medicine D, Nephrology, Hypertension and Rheumatology, University Hospital Muenster
Malte Lenders: Internal Medicine D, Nephrology, Hypertension and Rheumatology, University Hospital Muenster
Hermann J. Pavenstädt: Internal Medicine D, Nephrology, Hypertension and Rheumatology, University Hospital Muenster
Edwin Herrmann: Clinic for Urology, University Hospital Muenster
Stefan-Martin Brand: Institute of Sports Medicine, Molecular Genetics of Cardiovascular Disease, University Hospital Muenster
Eva Brand: Internal Medicine D, Nephrology, Hypertension and Rheumatology, University Hospital Muenster

DOI: https://doi.org/10.1186/s13148-017-0415-6
Journal volume & issue: Vol. 9, no. 1
pp. 1 – 10

Abstract

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Abstract Background KIBRA has been suggested as a key regulator of the Hippo signaling pathway, regulating organ size, cell contact inhibition, tissue regeneration as well as tumorigenesis and cystogenesis. We recently reported that human KIBRA expression depends on a complex alternative CpG-rich promoter system. Our current study aimed at the identification of epigenetic mechanisms associated with alterations in KIBRA expression regulation. Results We identified two separated methylation-sensitive CpG islands located to independent KIBRA promoter regions. In vitro promoter methylation analysis using human neuroblastoma (SH-SY5Y) and immortalized kidney cells (IHKE) revealed that total promoter methylation by CpG methyltransferase SssI resulted in complete abrogation of transcriptional activity (p < 0.001), while partial methylation by HpaII selectively repressed KIBRA core promoter activity in kidney cells (p < 0.001). Cell culture-based experiments demonstrated that 5-azacitidine may be used to restore KIBRA mRNA and protein levels, while overexpression of transcription factor SP1 also induced KIBRA upregulation (all p < 0.001). Furthermore, SP1 transactivation of KIBRA transcription was largely prevented by methylation of KIBRA regulatory elements (p < 0.001). Analysis of human kidney biopsies revealed that KIBRA promoter methylation was associated with human clear cell renal cell carcinoma (ccRCC; n = 8 vs 16 controls, OR = 1.921, [CI 95% = 1.369–2.695]). The subsequent determination of KIBRA mRNA levels by real-time PCR in a larger patient sample confirmed significantly reduced KIBRA expression in ccRCC (n = 32) compared to non-neoplastic human kidney tissue samples (controls, n = 32, p < 0.001). Conclusion We conclude that epigenetic downregulation of tumor suppressor KIBRA may involve impaired SP1 binding to functional methylation-sensitive KIBRA promoter elements as observed in human kidney clear cell carcinoma. Our findings provide a pathophysiological basis for future studies on altered KIBRA regulation in clinical disease entities such as renal cancer.

Published in Clinical Epigenetics

ISSN: 1868-7083 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine; Science: Biology (General): Genetics
Website: https://clinicalepigeneticsjournal.biomedcentral.com/

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