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Contribution of Kv4 channels toward the A-type potassium current in murine colonic myocytes

机译:鼠结肠肌细胞中Kv4通道对A型钾电流的贡献

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摘要

A rapidly inactivating K+ current (A-type current; IA) present in murine colonic myocytes is important in maintaining physiological patterns of slow wave electrical activity. The kinetic profile of colonic IA resembles that of Kv4-derived currents. We examined the contribution of Kv4 α-subunits to IA in the murine colon using pharmacological, molecular and immunohistochemical approaches. The divalent cation Cd2+ decreased peak IA and shifted the voltage dependence of activation and inactivation to more depolarized potentials. Similar results were observed with La3+. Colonic IA was sensitive to low micromolar concentrations of flecainide (IC50 = 11 μM). Quantitative PCR indicated that in colonic and jejunal tissue, Kv4.3 transcripts demonstrate greater relative abundance than transcripts encoding Kv4.1 or Kv4.2. Antibodies revealed greater Kv4.3-like immunoreactivity than Kv4.2-like immunoreactivity in colonic myocytes. Kv4-like immunoreactivity was less evident in jejunal myocytes. To address this finding, we examined the expression of K+ channel-interacting proteins (KChIPs), which act as positive modulators of Kv4-mediated currents. Qualitative PCR identified transcripts encoding the four known members of the KChIP family in isolated colonic and jejunal myocytes. However, the relative abundance of KChIP transcript was 2.6-fold greater in colon tissue than in jejunum, as assessed by quantitative PCR, with KChIP1 showing predominance. This observation is in accordance with the amplitude of the A-type current present in these two tissues, where colonic myocytes possess densities twice that of jejunal myocytes. From this we conclude that Kv4.3, in association with KChIP1, is the major molecular determinant of IA in murine colonic myocytes.
机译:鼠结肠肌细胞中存在的快速失活的K + 电流(A型电流; IA)对于维持慢波电活动的生理模式很重要。结肠IA的动力学曲线类似于Kv4衍生的电流。我们使用药理,分子和免疫组化方法检查了Kv4α亚基对鼠结肠中IA的贡献。二价阳离子Cd 2 + 降低了峰IA,并使活化和失活的电压依赖性转移到更多的去极化电位。 La 3 + 的结果相似。结肠IA对氟卡尼的低微摩尔浓度(IC50 = 11μM)敏感。定量PCR表明,在结肠和空肠组织中,Kv4.3转录物表现出比编码Kv4.1或Kv4.2的转录物更高的相对丰度。在结肠肌细胞中,抗​​体显示出比Kv4.2-样免疫反应性更高的Kv4.3-样免疫反应性。空肠肌细胞中Kv4样免疫反应性较弱。为了解决这一发现,我们检查了K + 通道相互作用蛋白(KChIPs)的表达,该蛋白可作为Kv4介导电流的正调节剂。定性PCR鉴定了在分离的结肠和空肠肌细胞中编码KChIP家族四个已知成员的转录本。然而,通过定量PCR评估,结肠组织中KChIP转录本的相对丰度比空肠高2.6倍,其中KChIP1占优势。该观察结果符合存在于这两个组织中的A型电流的幅度,其中结肠肌细胞的密度是空肠肌细胞的两倍。由此得出的结论是,Kv4.3与KChIP1结合是鼠结肠肌细胞中IA的主要分子决定因素。

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