Affiliation:
1. Department of Cardiology Heidelberg University Hospital Heidelberg Germany
2. DZHK (German Center for Cardiovascular Research) Partner Site Heidelberg/Mannheim University of Heidelberg Germany
3. HCR Heidelberg Center for Heart Rhythm Disorders Heidelberg University Hospital Heidelberg Germany
4. Digital Health Center Berlin Institute of Health (BIH) and Charité Berlin Germany
5. Department of Medical Oncology National Center for Tumor DiseasesHeidelberg University Hospital Heidelberg Germany
6. Health Data Science UnitMedical Faculty Heidelberg Heidelberg Germany
7. Department for Cardiology II: Electrophysiology University Hospital Münster Münster Germany
8. Department of Cardiac Surgery University of Heidelberg Germany
Abstract
Background
Atrial fibrillation (AF) is the most common sustained cardiac arrhythmia. However, underlying molecular mechanisms are insufficiently understood. Previous studies suggested that microRNA (miRNA) dependent gene regulation plays an important role in the initiation and maintenance of AF. The 2‐pore‐domain potassium channel TASK‐1 (tandem of P domains in a weak inward rectifying K
+
channel–related acid sensitive K
+
channel 1) is an atrial‐specific ion channel that is upregulated in AF. Inhibition of TASK‐1 current prolongs the atrial action potential duration to similar levels as in patients with sinus rhythm. Here, we hypothesize that miRNAs might be responsible for the regulation of
KCNK3
that encodes for TASK‐1.
Methods and Results
We selected miRNAs potentially regulating
KCNK3
and studied their expression in atrial tissue samples obtained from patients with sinus rhythm, paroxysmal AF, or permanent/chronic AF. MiRNAs differentially expressed in AF were further investigated for their ability to regulate
KCNK3
mRNA and TASK‐1 protein expression in human induced pluripotent stem cells, transfected with miRNA mimics or inhibitors. Thereby, we observed that miR‐34a increases TASK‐1 expression and current and further decreases the resting membrane potential of
Xenopus laevis
oocytes, heterologously expressing hTASK‐1. Finally, we investigated associations between miRNA expression in atrial tissues and clinical parameters of our patient cohort. A cluster containing AF stage, left ventricular end‐diastolic diameter, left ventricular end‐systolic diameter, left atrial diameter, atrial COL1A2 (collagen alpha‐2(I) chain), and TASK‐1 protein level was associated with increased expression of miR‐25, miR‐21, miR‐34a, miR‐23a, miR‐124, miR‐1, and miR‐29b as well as decreased expression of miR‐9 and miR‐485.
Conclusions
These results suggest an important pathophysiological involvement of miRNAs in the regulation of atrial expression of the TASK‐1 potassium channel in patients with atrial cardiomyopathy.
Publisher
Ovid Technologies (Wolters Kluwer Health)
Subject
Cardiology and Cardiovascular Medicine
Cited by
18 articles.
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