首页> 美国卫生研究院文献>The Journal of General Physiology >Distinct Transient Outward Potassium Current (Ito) Phenotypes and Distribution of Fast-inactivating Potassium Channel Alpha Subunits in Ferret Left Ventricular Myocytes
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Distinct Transient Outward Potassium Current (Ito) Phenotypes and Distribution of Fast-inactivating Potassium Channel Alpha Subunits in Ferret Left Ventricular Myocytes

机译:在雪貂左心室心肌细胞中的不同瞬时瞬态向外钾电流(Ito)表型和快速灭活钾通道α亚基的分布。

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摘要

The biophysical characteristics and α subunits underlying calcium-independent transient outward potassium current (Ito) phenotypes expressed in ferret left ventricular epicardial (LV epi) and endocardial (LV endo) myocytes were analyzed using patch clamp, fluorescent in situ hybridization (FISH), and immunofluorescent (IF) techniques. Two distinct Ito phenotypes were measured (21–22°C) in the majority of LV epi and LV endo myocytes studied. The two Ito phenotypes displayed marked differences in peak current densities, activation thresholds, inactivation characteristics, and recovery kinetics. Ito,epi recovered rapidly [τrec, −70 mV = 51 ± 3 ms] with minimal cumulative inactivation, while Ito,endo recovered slowly [τrec, −70 mV = 3,002 ± 447 ms] with marked cumulative inactivation. Heteropoda toxin 2 (150 nM) blocked Ito,epi in a voltage-dependent manner, but had no effect on Ito,endo. Parallel FISH and IF measurements conducted on isolated LV epi and LV endo myocytes demonstrated that Kv1.4, Kv4.2, and Kv4.3 α subunit expression in LV myocyte types was quite heterogenous: (a) Kv4.2 and Kv4.3 were more predominantly expressed in LV epi than LV endo myocytes, and (b) Kv1.4 was expressed in the majority of LV endo myocytes but was essentially absent in LV epi myocytes. In combination with previous measurements on recovery kinetics (Kv1.4, slow; Kv4.2/4.3, relatively rapid) and Heteropoda toxin block (Kv1.4, insensitive; Kv4.2, sensitive), our results strongly support the hypothesis that, in ferret heart, Kv4.2/Kv4.3 and Kv1.4 α subunits, respectively, are the molecular substrates underlying the Ito,epi and Ito,endo phenotypes. FISH and IF measurements were also conducted on ferret ventricular tissue sections. The three Ito α subunits again showed distinct patterns of distribution: (a) Kv1.4 was localized primarily to the apical portion of the LV septum, LV endocardium, and approximate inner 75% of the LV free wall; (b) Kv4.2 was localized primarily to the right ventricular free wall, epicardial layers of the LV, and base of the heart; and (c) Kv4.3 was localized primarily to epicardial layers of the LV apex and diffusely distributed in the LV free wall and septum. Therefore, in intact ventricular tissue, a heterogeneous distribution of candidate Ito α subunits not only exists from LV epicardium to endocardium but also from apex to base.
机译:使用膜片钳,荧光原位杂交(FISH)和分析了在雪貂左心室心外膜(LV epi)和心内膜(LV内膜)心肌中表达的钙独立的瞬时钙离子瞬时外向钾电流(Ito)表型的生物学特性和α亚基。免疫荧光(IF)技术。在研究的大多数LV Epi和LV内膜心肌细胞中,测量到两种不同的Ito表型(21–22°C)。这两种Ito表型在峰值电流密度,激活阈值,失活特性和恢复动力学方面显示出显着差异。 Ito,epi迅速恢复[τrec,-70 mV = 51±3 ms],累积失活最小,而Ito,endo缓慢恢复[τrec,-70 mV = 3,002±447 ms],累积失活明显。异足动物毒素2(150 nM)以电压依赖性方式阻断了Ito,epi,但对Ito,endo没有影响。对分离的LV Epi和LV内膜心肌细胞进行的平行FISH和IF测量表明,LV心肌细胞类型中的Kv1.4,Kv4.2和Kv4.3α亚基表达非常异质:(a)Kv4.2和Kv4.3在LV Epi中比在LV内皮细胞中更主要表达,并且(b)Kv1.4在大多数LV内皮细胞中表达,但在LV Epi心肌细胞中基本不存在。结合先前对恢复动力学(Kv1.4,慢; Kv4.2 / 4.3,相对快)和杂菌毒素阻滞(Kv1.4,不敏感; Kv4.2,敏感)的测量,我们的结果强烈支持以下假设:在雪貂心脏中,Kv4.2 / Kv4.3和K​​v1.4α亚基分别是Ito,epi和Ito,endo表型的分子底物。还对雪貂心室组织切片进行了FISH和IF测量。这三个Itoα亚基再次显示出不同的分布模式:(a)Kv1.4主要定位于LV间隔的顶端部分,LV心内膜和大约LV游离壁的内部75%; (b)Kv4.2主要定位于右心室游离壁,左心室心外膜层和心脏底部; (c)Kv4.3主要定位于LV顶点的心外膜层,并散布在LV自由壁和隔膜中。因此,在完整的心室组织中,候选Itoα亚基的异质分布不仅存在于左心外膜到心内膜,而且还存在于心尖到基部。

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