Non-neural electrical responses of smooth muscle cells of the rabbit basilar artery to electrical field stimulation.

Nagao, Toshiyasu; Suzuki, Hiroyoshi

doi:10.2170/jjphysiol.37.497

Cited by 15 publications

(13 citation statements)

References 33 publications

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“…In the basilar artery, multiple substances may be released during activation of endothelial cells, not only EDRF and EDHF but also endotheliumderived contracting factor (De Mey & Vanhoutte, 1983;Nagao & Suzuki, 1987) and also relaxing substances, such as prostacyclin (PGI2) (Moncada et al, 1977;Baenziger et al, 1977;Eldor et al, 1981;Domae & Kuriyama, 1986). It is unlikely that the effects of ACh on the guinea-pig basilar artery can be accounted for by the release of PGI2 since the relaxant response to ACh is unchanged by indomethacin and PGI2 does not hyperpolarize the membrane (unpublished observations).…”

Section: Discussionmentioning

confidence: 98%

Factors inducing endothelium‐dependent relaxation in the guinea‐pig basilar artery as estimated from the actions of haemoglobin

Nishiye¹,

Nakao²,

Itoh³

et al. 1989

British J Pharmacology

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1 Factors inducing dilatation of guinea-pig basilar artery were investigated in intact and endothelium-denuded tissues by measurement of isometric tension and by electrophysiological methods. 2 The amplitudes of contractions induced by 9,1 1,epithio-1 1,12-methanothromboxane A2 (STA2) and by high K+ were enhanced by haemoglobin (oxyhaemoglobin, Hb) in a concentrationdependent fashion (above 1 pM). For the high K'-induced contraction, the initial tonic component was enhanced to a greater extent than the secondary phasic component. Mechanical responses evoked by STA2 and by high K' were greater in endothelium-denuded tissues, but Hb (below 10pM) had no effect on them.3 Hb (10pM) had no effect on the contractile proteins as estimated from the actions of Hb on Ca2+-induced contractions in skinned muscle tissues. Further, Hb had no effect on the release of Ca2+ from intracellular stores but it accelerated the Ca2 + accumulation into the sarcoplasmic reticulum as judged from the caffeine-or STA2-induced contraction generated in intact tissues. 4 Acetylcholine (ACh) relaxed tissues that were precontracted by STA2 but Hb prevented this relaxation, in a concentration-dependent fashion. The ACh-induced relaxation was sustained for over 10min in the absence of Hb, but following application of Hb, ACh caused only a transient relaxation. 5 STA2 (up to 100nM) did not modify the resting membrane potential of smooth muscle cells of the basilar artery. ACh (1O pM) caused transient hyperpolarization which was only slightly inhibited by Hb (10pM) whether or not STA2 was present. The hyperpolarization induced by ACh required the presence of endothelial cells. 6 A23187 (0.01-1 pM) relaxed tissues which were precontracted by STA2, in a concentrationdependent fashion but had no effect on the membrane potential. 7 These results suggest that in guinea-pig basilar artery, ACh induces relaxation of tissues that were precontracted by STA2 by causing release of both endothelium-derived relaxing (EDRF) and endothelial dependent hyperpolarizing factor (EDHF) (sustained and initial transient relaxation, respectively), but via different mechanisms. Hb inhibits the former and to a lesser extent, the latter.Since A23187 produced relaxation of pre-contracted tissue but caused no detectable change in the membrane potential, this agent may release EDRF but not EDHF.

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Section: Discussionmentioning

confidence: 98%

Factors inducing endothelium‐dependent relaxation in the guinea‐pig basilar artery as estimated from the actions of haemoglobin

Nishiye¹,

Nakao²,

Itoh³

et al. 1989

British J Pharmacology

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“…As there are gap junctions between endothelial and adjacent smooth muscle cells (Rhodin, 1967;Taugner, Kirchheim & Forssmann, 1984), electrical coupling between these two types of cells may occur . In fact, the non-neuronal depolarizing responses elicited by electrical field stimulation in smooth muscle cells of the rabbit basilar artery are not generated after removal of the endothelium (Nagao & Suzuki, 1987). However, evidence that the hyperpolarization of smooth muscle cells in tissues with no endothelium can be produced indirectly (i.e.…”

Section: Discussionmentioning

confidence: 99%

Calcium dependency of the endothelium‐dependent hyperpolarization in smooth muscle cells of the rabbit carotid artery.

Chen

Suzuki

1990

The Journal of Physiology

146

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SUMMARY1. In smooth muscle cells of the rabbit carotid artery, ACh (> 10-8 M) generated a hyperpolarization with two components (transient followed by sustained), only in the tissues with an intact endothelium. There were no detectable changes in the membrane potential, as elicited by ACh (up to 10-5 M) in tissues with no endothelium or in the presence of atropine (10-6 M). 3. Procaine (> 10-6 M) inhibited the ACh-induced hyperpolarization in a concentration-dependent manner, and at a concentration of procaine (10-3 M) which caused substantial depolarization of the membrane, no detectable change was elicited by ACh.4. Caffeine (10-6_10-3 M) produced a transient hyperpolarization, independent of the presence or absence of the endothelium, and inhibited the sustained component of the ACh-induced hyperpolarization more so than the initial component. 5. A23187 (> 10-8 M) hyperpolarized the smooth muscle membrane in a concentration-dependent manner, and this hyperpolarization was not generated in Ca2+-free solution or in the absence of endothelial cells.6. In intact tissues, pre-treatment with A23187 resulted in a reduction of the subsequently generated ACh-induced hyperpolarization, in an irreversible manner.7. It would thus appear that in the rabbit carotid artery, the endotheliumdependent hyperpolarization induced by ACh has Ca2+-dependent and Ca2+-independent components, and each may be related to the increase in endothelial [Ca2+]i by release from the intracellular store and by influx from the extracellular medium, respectively. The increased [Ca2+], would trigger a release of an endothelium-derived hyperpolarizing factor (EDHF) from the endothelial cells.

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“…However, in the mechanically agitated bronchioles, almost all the examined sections (95%) had lost 60-90% of the epithelial luminal surface. We also used hypo-osmolarity shock to destroy the epithelial layer, as is done for endothelial cells in blood vessels (Bolton, Lang & Takewaki, 1984;Nagao & Suzuki, 1987). Histological examination of the bronchioles revealed that the epithelial luminal surface was completely destroyed after the hypo-osmolarity shock, as has been noted in blood vessels (Nagao & Suzuki, 1987).…”

Section: Methodsmentioning

confidence: 99%

“…The fixed needle was also used for electrical stimulation of ring preparations of the bronchiole. As required for the study, the epithelial cells were removed mechanically by rubbing the internal surface of the bronchioles with a fine silver wire (200 ,Im diameter) or by hypo-osmolarity shock by exposing the inner lumen of the bronchioles to distilled water for about 30-60 s as has previously been done in vascular tissues for removal of endothelial cells (Bolton et al 1984;Nagao & Suzuki, 1987).…”

Section: Methodsmentioning

confidence: 99%

Airway epithelial cells regulate membrane potential, neurotransmission and muscle tone of the dog airway smooth muscle.

Xie

Hakoda

Ito

1992

The Journal of Physiology

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SUMMARY1. The effects of epithelial cells were investigated on resting membrane potential and neuro-effector transmission in smooth muscle cells of the dog tracheal and bronchiolar tissues.2. The mean value of the resting membrane potential of the epithelium-intact bronchiolar smooth muscle cells of the dog was -700 + 1 mV (± S.D., n = 40) and mechanical denudation of the epithelial layer depolarized the membrane to -57 0 + 2'5 mV (± S.D., n = 40). Application of isolated and dispersed epithelial cells (> 2 x 105 cells/ml) to the perfusing solution repolarized the membrane of epithelium-denuded bronchiolar smooth muscle cells to -670 + 2-7 mV (± S.D., n = 20).The mean resting membrane potential of the mucosa-free tracheal smooth muscle cells was -59-1 + 1-4 mV (± S.D., n = 50), and application of isolated and dispersed cells (> 2 x 105 cells/ml) hyperpolarized the membrane to -67-2 + 1'8 mV (± S.D., n = 50). These repolarizing actions were not modified by indomethacin (10-5 M).3. In the epithelium-denuded bronchioles, ACh (> 10-9 M) dose-dependently depolarized the smooth muscle cells, while in the epithelium-intact bronchioles, ACh (10-11-10-8 M) did not affect the resting membrane potential. At a concentration of 10-7 M, ACh significantly depolarized the membrane.4. Electrical field stimulation (EFS; 50,ts in duration and about 10-20 V in strength) applied to ring preparations of the bronchioles evoked twitch-like contractions (hereafter referred as twitch contraction), and size of the twitch contractions gradually and continuously decreased in the presence or absence of indomethacin (10-5 M) and guanethidine (10-6 M). When similar experiments were performed using epithelium-denuded bronchiolar ring preparations, in no case was there a prominent reduction in the amplitude of the twitch contractions in the presence of indomethacin and guanethidine.5. The decremental response of the twitch contraction observed in the epitheliumintact bronchioles was overcome by application of the leukotriene synthesis inhibitor AA861 (10-6 M) and the leukotriene antagonist ON01078 (10-5 M).6. Leukotrienes C4 and D4 (LTC4 and LTD4, > 10-8 M) evoked muscle contraction with a steady increase in muscle tone, up to a certain level. However, at 10-9 M, LTC4 increased and LTD4 decreased the amplitude of the twitch contractions evoked by MS 9432

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Non-neural electrical responses of smooth muscle cells of the rabbit basilar artery to electrical field stimulation.

Cited by 15 publications

References 33 publications

Factors inducing endothelium‐dependent relaxation in the guinea‐pig basilar artery as estimated from the actions of haemoglobin

Factors inducing endothelium‐dependent relaxation in the guinea‐pig basilar artery as estimated from the actions of haemoglobin

Calcium dependency of the endothelium‐dependent hyperpolarization in smooth muscle cells of the rabbit carotid artery.

Airway epithelial cells regulate membrane potential, neurotransmission and muscle tone of the dog airway smooth muscle.

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