MicroRNA Expression in Alpha and Beta Cells of Human Pancreatic Islets | Zendy

Dagmar Klein | Zendy; Ryosuke Misawa | Zendy; Valia Bravo-Egaña | Zendy; Nancy Vargas | Zendy; Samuel Rosero | Zendy; Julieta Piroso | Zendy; Hirohito Ichii | Zendy; Oliver Umland | Zendy; Zhijie Jiang | Zendy; Nicholas F. Tsinoremas | Zendy; Camillo Ricordi | Zendy; Luca Inverardi | Zendy; Juan DomínguezBendala | Zendy; Ricardo L. Pastori | Zendy

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MicroRNA Expression in Alpha and Beta Cells of Human Pancreatic Islets

Author(s) -

Dagmar Klein,

Ryosuke Misawa,

Valia Bravo-Egaña,

Nancy Vargas,

Samuel Rosero,

Julieta Piroso,

Hirohito Ichii,

Oliver Umland,

Zhijie Jiang,

Nicholas F. Tsinoremas,

Camillo Ricordi,

Luca Inverardi,

Juan DomínguezBendala,

Ricardo L. Pastori

Publication year - 2013

Publication title -

plos one

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.99

H-Index - 332

ISSN - 1932-6203

DOI - 10.1371/journal.pone.0055064

Subject(s) - microrna , biology , gene expression , gene expression profiling , microbiology and biotechnology , cell sorting , regulation of gene expression , flow cytometry , alpha cell , cell culture , pancreatic islets , beta cell , gene , islet , genetics , endocrinology , insulin

microRNAs (miRNAs) play an important role in pancreatic development and adult β-cell physiology. Our hypothesis is based on the assumption that each islet cell type has a specific pattern of miRNA expression. We sought to determine the profile of miRNA expression in α-and β-cells, the main components of pancreatic islets, because this analysis may lead to a better understanding of islet gene regulatory pathways. Highly enriched (>98%) subsets of human α-and β-cells were obtained by flow cytometric sorting after intracellular staining with c-peptide and glucagon antibody. The method of sorting based on intracellular staining is possible because miRNAs are stable after fixation. MiRNA expression levels were determined by quantitative high throughput PCR-based miRNA array platform screening. Most of the miRNAs were preferentially expressed in β-cells. From the total of 667 miRNAs screened, the Significant Analysis of Microarray identified 141 miRNAs, of which only 7 were expressed more in α-cells (α-miRNAs) and 134 were expressed more in β-cells (β-miRNAs). Bioinformatic analysis identified potential targets of β-miRNAs analyzing the Beta Cell Gene Atlas, described in the T1Dbase, the web platform, supporting the type 1 diabetes (T1D) community. cMaf, a transcription factor regulating glucagon expression expressed selectively in α-cells (TFα) is targeted by β-miRNAs; miR-200c, miR-125b and miR-182. Min6 cells treated with inhibitors of these miRNAs show an increased expression of cMaf RNA. Conversely, over expression of miR-200c, miR-125b or miR-182 in the mouse alpha cell line αTC6 decreases the level of cMAF mRNA and protein. MiR-200c also inhibits the expression of Zfpm2, a TFα that inhibits the PI3K signaling pathway, at both RNA and protein levels. In conclusion, we identified miRNAs differentially expressed in pancreatic α- and β-cells and their potential transcription factor targets that could add new insights into different aspects of islet biology and pathophysiology.

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