Dual role of miR-1 in the development and function of sinoatrial cells

Dual role of miR-1 in the development and function of sinoatrial cells

miR-1, the most abundant miRNA in the heart, modulates expression of several transcription factors and ion channels. Conditions affecting the heart rate, such as endurance training and cardiac diseases, show a concomitant miR-1 up- or down-regulation. Here, we investigated the role of miR-1 overexpr...

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Veröffentlicht in:Journal of molecular and cellular cardiology 2021-08, Vol.157, p.104-112
Hauptverfasser: Benzoni, P., Nava, L., Giannetti, F., Guerini, G., Gualdoni, A., Bazzini, C., Milanesi, R., Bucchi, A., Baruscotti, M., Barbuti, A.
Format: Artikel
Sprache:eng
Schlagworte:
Action Potentials
Activated-Leukocyte Cell Adhesion Molecule - metabolism
Animals
Biomarkers
Cardiac & Cardiovascular Systems
Cardiovascular System & Cardiology
Cell Biology
Cell Differentiation - genetics
Electrophysiological Phenomena
Embryonic stem cells
Embryonic Stem Cells - cytology
Embryonic Stem Cells - metabolism
Gene Expression
Gene Expression Regulation
HCN4
If current
Immunophenotyping
Life Sciences & Biomedicine
Mice
microRNA
MicroRNAs - genetics
miR-1
Myocytes, Cardiac - cytology
Myocytes, Cardiac - metabolism
Rats
Science & Technology
Sinoatrial Node - cytology
Sinoatrial Node - metabolism
Sinus node
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Zusammenfassung:miR-1, the most abundant miRNA in the heart, modulates expression of several transcription factors and ion channels. Conditions affecting the heart rate, such as endurance training and cardiac diseases, show a concomitant miR-1 up- or down-regulation. Here, we investigated the role of miR-1 overexpression in the development and function of sinoatrial (SAN) cells using murine embryonic stem cells (mESC). We generated mESCs either overexpressing miR-1 and EGFP (miR1OE) or EGFP only (EM). SAN-like cells were selected from differentiating mESC using the CD166 marker. Gene expression and electrophysiological analysis were carried out on both early mES-derived cardiac progenitors and SAN-like cells and on beating neonatal rat ventricular cardiomyocytes (NRVC) over-expressing miR-1. miR1OE cells increased significantly the proportion of CD166+ SAN precursors compared to EM cells (23% vs 12%) and the levels of the transcription factors TBX5 and TBX18, both involved in SAN development. miR1OE SAN-like cells were bradycardic (1,3 vs 2 Hz) compared to EM cells. In agreement with data on native SAN cells, EM SAN-like cardiomyocytes show two populations of cells expressing either slow- or fast-activating If currents; miR1OE SAN-like cells instead have only fast-activating If with a significantly reduced conductance. Western Blot and immunofluorescence analysis showed a reduced HCN4 signal in miR-1OE vs EM CD166+ precursors. Together these data point out to a specific down-regulation of the slow-activating HCN4 subunit by miR-1. Importantly, the rate and If alterations were independent of the developmental effects of miR-1, being similar in NRVC transiently overexpressing miR-1. In conclusion, we demonstrated a dual role of miR-1, during development it controls the proper development of sinoatrial-precursor, while in mature SAN-like cells it modulates the HCN4 pacemaker channel translation and thus the beating rate. [Display omitted] •miR-1 increase SAN-specific transcription factors and the number of SAN precursors during sinus node development•Silencing miR-1 impair spontaneous contraction in mESC-derived embryoid bodies.•miR-1 slows the beating rate of pacemaker cells by inhibiting HCN4 translation and thus reducing the If current•miR-1 Overexpression accelerate If activation kinetics and decreases cAMP response compatibly with a decreased HCN4/HCN1
ISSN:0022-2828
1095-8584
DOI:10.1016/j.yjmcc.2021.05.001