MiRNA-149 as a Candidate for Facial Clefting and Neural Crest Cell Migration

生物 神经嵴 候选基因 小RNA 遗传学 诱导多能干细胞 表型 转录组 全基因组关联研究 生物信息学 基因 基因表达 胚胎干细胞 单核苷酸多态性 基因型
作者
L G Stüssel,Ronja Hollstein,Magdalena Laugsch,Lara M. Hochfeld,Julia Welzenbach,Julia Schröder,Frederic Thieme,Nina Ishorst,Rosario Romero,Leonie Weinhold,Timo Hess,Jan Gehlen,Adrianna Mostowska,Stefanie Heilmann‐Heimbach,Elisabeth Mangold,Álvaro Rada-Iglesias,Michael Knapp,Christian P. Schaaf,Kerstin U. Ludwig
出处
期刊:Journal of Dental Research [SAGE Publishing]
卷期号:101 (3): 323-330 被引量:4
标识
DOI:10.1177/00220345211038203
摘要

Nonsyndromic cleft lip with or without palate (nsCL/P) ranks among the most common human birth defects and has a multifactorial etiology. Human neural crest cells (hNCC) make a substantial contribution to the formation of facial bone and cartilage and are a key cell type in terms of nsCL/P etiology. Based on increasing evidence for the role of noncoding regulatory mechanisms in nsCL/P, we investigated the role of hNCC-expressed microRNAs (miRNA) in cleft development. First, we conducted a systematic analysis of miRNAs expressed in human-induced pluripotent stem cell-derived hNCC using Affymetrix microarrays on cell lines established from 4 unaffected donors. These analyses identified 152 candidate miRNAs. Based on the hypothesis that candidate miRNA loci harbor genetic variation associated with nsCL/P risk, the genomic locations of these candidates were cross-referenced with data from a previous genome-wide association study of nsCL/P. Associated variants were reanalyzed in independent nsCL/P study populations. Jointly, the results suggest that miR-149 is implicated in nsCL/P etiology. Second, functional follow-up included in vitro overexpression and inhibition of miR-149 in hNCC and subsequent analyses at the molecular and phenotypic level. Using 3'RNA-Seq, we identified 604 differentially expressed (DE) genes in hNCC overexpressing miR-149 compared with untreated cells. These included TLR4 and JUNB, which are established targets of miR-149, and NOG, BMP4, and PAX6, which are reported nsCL/P candidate genes. Pathway analyses revealed that DE genes were enriched in pathways including regulation of cartilage development and NCC differentiation. At the cellular level, distinct hNCC migration patterns were observed in response to miR-149 overexpression. Our data suggest that miR-149 is involved in the etiology of nsCL/P via its role in hNCC migration.

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