Characterization of Stimulatory Action on Voltage-Gated Na+ Currents Caused by Omecamtiv Mecarbil, Known to Be a Myosin Activator

Chih-Yu Ting; Chia-Lung Shih; Meng-Cheng Yu; Chao-Liang Wu; Sheng-Nan Wu

doi:10.3390/biomedicines11051351

Characterization of Stimulatory Action on Voltage-Gated Na⁺ Currents Caused by Omecamtiv Mecarbil, Known to Be a Myosin Activator

Biomedicines. 2023 May 3;11(5):1351. doi: 10.3390/biomedicines11051351.

Authors

Chih-Yu Ting¹, Chia-Lung Shih², Meng-Cheng Yu³, Chao-Liang Wu², Sheng-Nan Wu^{3

4}

Affiliations

¹ Department of Emergency Medicine, Ditmanson Medical Foundation Chia-Yi Christian Hospital, Chiayi City 60002, Taiwan.
² Clinical Research Center, Ditmanson Medical Foundation Chia-Yi Christian Hospital, Chiayi City 60002, Taiwan.
³ Department of Physiology, National Cheng Kung University Medical College, Tainan 70101, Taiwan.
⁴ School of Medicine, National Sun Yat-Sen University College of Medicine, Kaohsiung 80424, Taiwan.

Abstract

Omecamtiv mecarbil (OM, CK-1827452) is recognized as an activator of myosin and has been demonstrated to be beneficial for the treatment of systolic heart failure. However, the mechanisms by which this compound interacts with ionic currents in electrically excitable cells remain largely unknown. The objective of this study was to investigate the effects of OM on ionic currents in GH3 pituitary cells and Neuro-2a neuroblastoma cells. In GH₃ cells, whole-cell current recordings showed that the addition of OM had different potencies in stimulating the transient (I_Na(T)) and late components (I_Na(L)) of the voltage-gated Na⁺ current (I_Na) with different potencies in GH₃ cells. The EC₅₀ value required to observe the stimulatory effect of this compound on I_Na(T) or I_Na(L) in GH₃ cells was found to be 15.8 and 2.3 µM, respectively. Exposure to OM did not affect the current versus voltage relationship of I_Na(T). However, the steady-state inactivation curve of the current was observed to shift towards a depolarized potential of approximately 11 mV, with no changes in the slope factor of the curve. The addition of OM resulted in an increase in the decaying time constant during the cumulative inhibition of I_Na(T) in response to pulse-train depolarizing stimuli. Furthermore, the presence of OM led to a shortening of the recovery time constant in the slow inactivation of I_Na(T). Adding OM also resulted in an augmentation of the strength of the window Na⁺ current, which was evoked by a short ascending ramp voltage. However, the OM exposure had little to no effect on the magnitude of L-type Ca²⁺ currents in GH₃ cells. On the other hand, the delayed-rectifier K⁺ currents in GH₃ cells were observed to be mildly suppressed in its presence. Neuro-2a cells also showed a susceptibility to the differential stimulation of I_Na(T) or I_Na(L) upon the addition of OM. Molecular analysis revealed potential interactions between the OM molecule and hNa_V1.7 channels. Overall, the direct stimulation of I_Na(T) and I_Na(L) by OM is assumed to not be mediated by an interaction with myosin, and this has potential implications for its pharmacological or therapeutic actions occurring in vivo.

Keywords: cumulative inactivation; late Na+ current; myosin activator; omecamtiv mecarbil; slow inactivation; transient Na+ current; voltage-gated Na+ current; window Na+ current.

Abstract

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