Abstract

Recently, we have identified a novel Ca2+-activated K+ current (Ik,ca) in human and mouse atrial myocytes that contributes markedly towards the late phase of the atrial repolarization. The importance of the currents is underpinned by the fact that the late phase of the cardiac action potential is susceptible to aberrant excitation e.g. early after depolarization and arrhythmias. The channel is differentially expressed in atrial vs. ventricular myocytes. Finally, we have preliminary data, which suggest that the channel may co-localize with specific isoform of the voltage-gated Ca 2+ channels (VGCC). We hypothesize that the regional specific expression of the Ca 2+-activated K + channels (Kca) coordinates distinct functional roles in atria vs. ventricles. Specifically, we hypothesize that the channels are important in the repolarization process in atria, and alteration of the current can precipitate profound changes in the shape and duration of cardiac action potentials and possibly atrial arrhythmias. The following Specific Aims are proposed: 1. Functional identification of Ik, ca, in atrial and ventricular myocytes. We will determine the detail biophysical and pharmacologic properties of Ik,ca as well as quantifying the whole-cell current density in human and mouse myocytes to define the specific isoforms of Ik,ca, expressed in atria and ventricles. To conclusively establish that the activity of Ik,ca contributes towards the repolarization process in the heart, we will employ in-vitro adenoviral-mediated gene transfer to single isolated human and mouse cardiac myocytes using dominant-negative (DN) functional knockout strategies. 2. Biochemical identification of the specific isoform encoding the cardiac Ik,ca, The functional study will be corroborated using Western blot analysis, ribonuclease protection assay (RPA), reverse transcriptase-polymerase chain reaction (RT-PCR), immunofluorescence techniques and in-situ hybridization. 3. Co-localization of cardiac Kca, channel with specific isoform of VGCC. To test the hypothesis that the channel colocalizes with specific isoform of VGCC, immunofluorescence techniques using double labeling will be used. In addition, we will use a gene targeted eqD Ca2+ channel null mutant mice as a tool to specifically examine the co-localization of the Kca channel with the different isoforms of VGCC. 4. Determination of the functional roles of Ik,ca in whole animals. In-vivo adenoviral-mediated gene transfer to overexpress the functional Kca channel or engineered DN constructs to mice and in vivo electrophysiologic studies will be used to assess the functional roles of the channel in whole animals. Complimentary experiments using transgenic mice of specific SK channel will be performed. Transgenic mice with conditional expression for each of the three SK channel genes have already been constructed. These mouse models will be used to study the functional roles of the Kca channel in the heart. ECG, telemetric ECG recordings and electrophysiologic studies will be performed. Single isolated myocytes will be studied using patch-clamp techniques as in Aim 1.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL075274-02
Application #
6919301
Study Section
Special Emphasis Panel (ZRG1-CVS-G (02))
Program Officer
Przywara, Dennis
Project Start
2004-07-01
Project End
2008-06-30
Budget Start
2005-07-01
Budget End
2006-06-30
Support Year
2
Fiscal Year
2005
Total Cost
$371,250
Indirect Cost

  Institution

Name
University of California Davis
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
047120084
City
Davis
State
CA
Country
United States
Zip Code
95618

  Publications

López, Javier E; Sharma, Janhavi; Avila, Jorge et al. (2017) Novel large-particle FACS purification of adult ventricular myocytes reveals accumulation of myosin and actin disproportionate to cell size and proteome in normal post-weaning development. J Mol Cell Cardiol 111:114-122
Myers, Richard; Timofeyev, Valeriy; Li, Ning et al. (2015) Feedback mechanisms for cardiac-specific microRNAs and cAMP signaling in electrical remodeling. Circ Arrhythm Electrophysiol 8:942-50
Lu, Ling; Sirish, Padmini; Zhang, Zheng et al. (2015) Regulation of gene transcription by voltage-gated L-type calcium channel, Cav1.3. J Biol Chem 290:4663-76
Jian, Zhong; Han, Huilan; Zhang, Tieqiao et al. (2014) Mechanochemotransduction during cardiomyocyte contraction is mediated by localized nitric oxide signaling. Sci Signal 7:ra27
Liu, Jun-Yan; Lin, Yan-Ping; Qiu, Hong et al. (2013) Substituted phenyl groups improve the pharmacokinetic profile and anti-inflammatory effect of urea-based soluble epoxide hydrolase inhibitors in murine models. Eur J Pharm Sci 48:619-27
Glatter, Kathryn A; Myers, Richard; Chiamvimonvat, Nipavan (2012) Recommendations regarding dietary intake and caffeine and alcohol consumption in patients with cardiac arrhythmias: what do you tell your patients to do or not to do? Curr Treat Options Cardiovasc Med 14:529-35
Zhang, Qian; Timofeyev, Valeriy; Qiu, Hong et al. (2011) Expression and roles of Cav1.3 (ýý1D) L-type Caýý+ channel in atrioventricular node automaticity. J Mol Cell Cardiol 50:194-202
Li, Ning; Liu, Jun-Yan; Qiu, Hong et al. (2011) Use of metabolomic profiling in the study of arachidonic acid metabolism in cardiovascular disease. Congest Heart Fail 17:42-6
Tuteja, Dipika; Rafizadeh, Sassan; Timofeyev, Valeriy et al. (2010) Cardiac small conductance Ca2+-activated K+ channel subunits form heteromultimers via the coiled-coil domains in the C termini of the channels. Circ Res 107:851-9
Li, Ning; Timofeyev, Valeriy; Tuteja, Dipika et al. (2009) Ablation of a Ca2+-activated K+ channel (SK2 channel) results in action potential prolongation in atrial myocytes and atrial fibrillation. J Physiol 587:1087-100

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