Rhythmic Ryanodine Receptor Ca
            <sup>2+</sup>
            Releases During Diastolic Depolarization of Sinoatrial Pacemaker Cells Do Not Require Membrane Depolarization

Vinogradova, Tatiana M.; Zhou, Ying; Maltsev, Victor A.; Lyashkov, Alexey E.; Stern, Michael D.; Lakatta, Edward G.

doi:10.1161/01.res.0000122045.55331.0f

Cited by 159 publications

(253 citation statements)

References 35 publications

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“…In the present context, the evidence indicates that overdrive increases force and rate through the generally agreed [3][4][5][6] increase in cellular calcium. Furthermore, in high [K + ] o overdrive is shown to simultaneously increase the twitch and the size as well as slope of diastolic potential which then subside together during recovery ( Figure 10).…”

Section: Calcium Load and Dominant Dischargesupporting

confidence: 52%

“…It is generally agreed that force development is a function of Ca 2+ loading [see 5,34]: indeed, an increase in rate increases cellular Ca 2+ in all cardiac tissues including the SAN (e.g., [3][4][5][6]. Also, overdrive-induced force patterns in SAN are similar to those in other cardiac tissues (e.g., [2,7]).…”

Section: Overdrive Increased Calcium Load and Forcementioning

confidence: 99%

“…It entails an enhanced ion exchange between extraand intra-cellular environments, since the number of action potentials increases in the unit of time. Indeed, a faster rate increases intracellular Na + [1,2] and Ca 2+ [e.g., [3][4][5] in cardiac tissues, including the SAN [6]. Overdrive increases contractile force as well [e.g., 5,7].…”

Section: Introductionmentioning

confidence: 99%

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Mechanisms underlying overdrive suppression and overdrive excitation in guinea pig sino-atrial node

Vassalle

2006

J Biomed Sci

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SummaryThe hypothesis that the pause that follows overdrive of the sino-atrial node (SAN) might be the net result of overdrive excitation and overdrive suppression was tested by studying rate and force patterns induced by overdrive in isolated guinea pig SAN superfused in vitro. In Tyrode solution, the pause is short and changes but little with longer or faster drives. increases the rate as well as it shortens the pause, whereas Ni 2+ decreases force as well as rate and lengthens the pause. Barium dissociates the effects on force and rate. Lidocaine and tetrodotoxin decrease rate and force, and increase the pause duration. In overdrive excitation, the increase in rate is associated with an enhancement of diastolic voltage oscillations. It is concluded that in SAN the prevalence of Ca 2+ load leads to overdrive excitation whereas the prevalence of Na + load leads to overdrive suppression. In Tyrode solution, the pause after drive appears to be the net result of these two different mechanisms.Abbreviations: AP -action potential; MDP -maximum diastolic potential; DD -diastolic depolarization; R -control rate (prior to drive); F -control contractile force; DF 1 -force of first driven beat; DF 2 -force of last driven beat; pause -time interval between the last driven beat and the first spontaneous beat; PDF 1 -force of the first beat after the pause; PDR 1 -rate immediately after the pause; PDR 2 -late (10-15 s) postdrive rate; PDF 2 -late (10-15 s) post-drive force (see Figure 1); SR -sarcoplasmic reticulum; g K -K + conductance; a i Na -intracellular Na + activity; TTX -tetrodotoxin; NCX -Na + -Ca 2+ exchange current

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Section: Calcium Load and Dominant Dischargesupporting

confidence: 52%

Section: Overdrive Increased Calcium Load and Forcementioning

confidence: 99%

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Mechanisms underlying overdrive suppression and overdrive excitation in guinea pig sino-atrial node

Vassalle

2006

J Biomed Sci

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“…The speed at which the Ca 2+ clock runs is assessed by the LCR period, defined as the time from the AP-induced Ca 2+ transient early in the cycle (Fig.1A, Clock "reset", blue) to LCR emergence during the subsequent DD (Clock "tick"). This Ca 2+ clock's period is slightly shorter than the cycle length (Fig.1A) and approximately coincides with the period of the intrinsic Ca 2+ oscillations under voltage clamp [27,30]. The speed at which Ca 2+ clock ticks is variable, matching the chronotropic demand for a given condition, and is governed by the SR Ca 2+ loading and Ca 2+ release characteristics, which in turn, are governed by the degree of phosphorylation of its aforementioned Ca 2+ cycling proteins.…”

Section: Ca 2+ Cycling Within Cardiac Pacemaker Cells Is a "Clock"mentioning

confidence: 59%

“…The net effects of this phosphorylation create conditions that are required for LCR spontaneous activation during the DD. The LCR activation in rabbit SANC is indeed truly spontaneous as it does not depend on membrane depolarization (but see [29] for cat latent atrial pacemaker cells), and can be observed under voltage clamp or in permeabilized SANC [27,30]. Importantly, it is the spontaneous emergence of LCRs during the late DD that activates I NCX and thus changes the DD dynamics from a linear to a nonlinear, exponentially rising function, culminating in I CaL activation and membrane excitation (Fig.1A) [17,18].…”

Section: How Cell Ca 2+ Cycling Links To Ncx Function and Why It Is Cmentioning

confidence: 99%

Cardiac pacemaker cell failure with preserved If, ICaL, and IKr: A lesson about pacemaker function learned from ischemia-induced bradycardia

Maltsev

Lakatta

2007

Journal of Molecular and Cellular Cardiology

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Cardiac ischemia is an important global health problem. It leads to contraction failure, arrhythmias, and cardiac cell death. Sinus bradycardia characterized by a slow heart rate (<60 bpm) is a prominent ischemia-related arrhythmia directly caused by a deficiency of heart beat initiation within the sinoatrial node (SAN), due to a failure of the heart's primary pacemaker cells (SANC). The study presented by Yi-Mei Du and Richard Nathan in this issue of Journal of Molecular and Cellular Cardiology [1] deals with the ionic basis of ischemia-induced bradycardia in isolated SANC. The results of their study not only contribute to understanding of ischemia-induced bradycardia, but also help to delineate the fundamental mechanisms of cardiac pacemaker cell function. Study design and hypothesisIn their studies, Du and Nathan simulated ischemia by superfusing SANC with a solution without glucose, at pH 6.6 that contained either 5.4 or 10 mM KCl. This lead, to a 13% or 43% reduction, respectively, in the spontaneous beating rate of freshly isolated SANC. This simulated ischemia is not true ischemia, e.g. there is no associated hypoxia or flow deficiency effects other than elevated [K + ]. Nonetheless simulated ischemia of this sort is often applied in studies like the present one. And, in their careful approach to the problem, the authors first demonstrated that their "ischemic" solutions produced bradycardia in the intact rabbit heart. Then, in isolated SANC they measured the effects of this simulated ischemia on membrane potential and ion currents under voltage clamp. Such an approach is not surprising, because it has been believed for almost half a century that the heart rhythm originates on the surface membrane of the cardiac pacemaker cells. This dogma stems from the Nobel prize triumph of the Hodgkin-Huxley neuron membrane excitability theory [2] and subsequent modification of this theory and extrapolation to the heart cells by Noble (1960) [3]. According to this theory, generation of spontaneous action potentials (APs) by cardiac pacemaker cells is portrayed as a membrane delimited process, i.e. by a pure interplay of time-and voltage-dependent ion currents. Pacemaker field researchers have focused mainly on the identification of multiple ion current components in pacemaker cells, and their respective roles in the spontaneous diastolic depolarization of these cells (DD, Fig.1A) that brings the membrane to the excitation threshold (reviews [4,5]). Du and Nathan thus tested an hypothesis that bradycardia induced by their

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Integrative modeling of the cardiac ventricular myocyte

Winslow

Cortassa

O’Rourke

et al. 2010

WIREs Mechanisms of Disease

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Cardiac electrophysiology is a discipline with a rich 50-year history of experimental research coupled with integrative modeling which has enabled us to achieve a quantitative understanding of the relationships between molecular function and the integrated behavior of the cardiac myocyte in health and disease. In this paper, we review the development of integrative computational models of the cardiac myocyte. We begin with a historical overview of key cardiac cell models that helped shape the field. We then narrow our focus to models of the cardiac ventricular myocyte and describe these models in the context of their subcellular functional systems including dynamic models of voltage-gated ion channels, mitochondrial energy production, ATP-dependent and electrogenic membrane transporters, intracellular Ca dynamics, mechanical contraction, and regulatory signal transduction pathways. We describe key advances and limitations of the models as well as point to new directions for future modeling research.

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Rhythmic Ryanodine Receptor Ca ²⁺ Releases During Diastolic Depolarization of Sinoatrial Pacemaker Cells Do Not Require Membrane Depolarization

Cited by 159 publications

References 35 publications

Mechanisms underlying overdrive suppression and overdrive excitation in guinea pig sino-atrial node

Mechanisms underlying overdrive suppression and overdrive excitation in guinea pig sino-atrial node

Cardiac pacemaker cell failure with preserved If, ICaL, and IKr: A lesson about pacemaker function learned from ischemia-induced bradycardia

Integrative modeling of the cardiac ventricular myocyte

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Rhythmic Ryanodine Receptor Ca 2+ Releases During Diastolic Depolarization of Sinoatrial Pacemaker Cells Do Not Require Membrane Depolarization

Cited by 159 publications

References 35 publications

Mechanisms underlying overdrive suppression and overdrive excitation in guinea pig sino-atrial node

Mechanisms underlying overdrive suppression and overdrive excitation in guinea pig sino-atrial node

Cardiac pacemaker cell failure with preserved If, ICaL, and IKr: A lesson about pacemaker function learned from ischemia-induced bradycardia

Integrative modeling of the cardiac ventricular myocyte

Contact Info

Product

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Rhythmic Ryanodine Receptor Ca ²⁺ Releases During Diastolic Depolarization of Sinoatrial Pacemaker Cells Do Not Require Membrane Depolarization