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Identification of differentially expressed miRNAs associated with chronic kidney disease-mineral bone disorder

Authors
Kim, Kyung ImJeong, SohyunHan, NayoungOh, Jung MiOh, Kook-HwanKim, In-Wha
Issue Date
Sep-2017
Publisher
SPRINGER
Keywords
chronic kidney disease; microRNA; mineral bone disorder; uremia
Citation
FRONTIERS OF MEDICINE, v.11, no.3, pp.378 - 385
Indexed
SCIE
SCOPUS
Journal Title
FRONTIERS OF MEDICINE
Volume
11
Number
3
Start Page
378
End Page
385
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/82414
DOI
10.1007/s11684-017-0541-8
ISSN
2095-0217
Abstract
The purpose of this study is to characterize a meta-signature of differentially expressed mRNA in chronic kidney disease (CKD) to predict putative microRNA (miRNA) in CKD-mineral bone disorder (CKD-MBD) and confirm the changes in these genes and miRNA expression under uremic conditions by using a cell culture system. PubMed searches using MeSH terms and keywords related to CKD, uremia, and mRNA arrays were conducted. Through a computational analysis, a meta-signature that characterizes the significant intersection of differentially expressed mRNA and expected miRNAs associated with CKD-MBD was determined. Additionally, changes in gene and miRNA expressions under uremic conditions were confirmed with human Saos-2 osteoblast-like cells. A statistically significant mRNA meta-signature of upregulated and downregulated mRNA levels was identified. Furthermore, miRNA expression profiles were inferred, and computational analyses were performed with the imputed microRNA regulation based on weighted ranked expression and putative microRNA targets (IMRE) method to identify miRNAs associated with CKD occurrence. TLR4 and miR-146b levels were significantly associated with CKD-MBD. TLR4 levels were significantly downregulated, whereas primiR- 146b and miR-146b were upregulated in the presence of uremic toxins in human Saos-2 osteoblast-like cells. Differentially expressed miRNAs associated with CKD-MBD were identified through a computational analysis, and changes in gene and miRNA expressions were confirmed with an in vitro cell culture system.
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