DNA Methyltransferase 1 Controls Nephron Progenitor Cell Renewal and Differentiation

生物 DNA甲基化 肾单位 DNMT1型 DNA甲基转移酶 甲基转移酶 细胞生物学 癌症研究 甲基化 遗传学 基因表达 DNA 基因
作者
Nicola Wanner,Julia Vornweg,Alexander N. Combes,Sean B. Wilson,Julia Plappert,Gesa Rafflenbeul,Victor G. Puelles,Raza‐Ur Rahman,Timur Liwinski,Saskia Lindner,Florian Grahammer,Oliver Kretz,Mary E. Wlodek,Tania Romano,Karen M. Moritz,Melanie Boerries,Hauke Busch,Stefan Bonn,Melissa H. Little,Wibke Bechtel‐Walz,Tobias B. Huber
出处
期刊:Journal of The American Society of Nephrology 卷期号:30 (1): 63-78 被引量:58
标识
DOI:10.1681/asn.2018070736
摘要

Background Nephron number is a major determinant of long-term renal function and cardiovascular risk. Observational studies suggest that maternal nutritional and metabolic factors during gestation contribute to the high variability of nephron endowment. However, the underlying molecular mechanisms have been unclear. Methods We used mouse models, including DNA methyltransferase ( Dnmt1, Dnmt3a, and Dnmt3b ) knockout mice, optical projection tomography, three-dimensional reconstructions of the nephrogenic niche, and transcriptome and DNA methylation analysis to characterize the role of DNA methylation for kidney development. Results We demonstrate that DNA hypomethylation is a key feature of nutritional kidney growth restriction in vitro and in vivo, and that DNA methyltransferases Dnmt1 and Dnmt3a are highly enriched in the nephrogenic zone of the developing kidneys. Deletion of Dnmt1 in nephron progenitor cells (in contrast to deletion of Dnmt3a or Dnm3b ) mimics nutritional models of kidney growth restriction and results in a substantial reduction of nephron number as well as renal hypoplasia at birth. In Dnmt1 -deficient mice, optical projection tomography and three-dimensional reconstructions uncovered a significant reduction of stem cell niches and progenitor cells. RNA sequencing analysis revealed that global DNA hypomethylation interferes in the progenitor cell regulatory network, leading to downregulation of genes crucial for initiation of nephrogenesis, Wt1 and its target Wnt4. Derepression of germline genes, protocadherins, Rhox genes, and endogenous retroviral elements resulted in the upregulation of IFN targets and inhibitors of cell cycle progression. Conclusions These findings establish DNA methylation as a key regulatory event of prenatal renal programming, which possibly represents a fundamental link between maternal nutritional factors during gestation and reduced nephron number.
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