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超分辨率扫描膜片钳技术揭示成年心室肌细胞功能性离子通道的簇集现象。

Super-resolution scanning patch clamp reveals clustering of functional ion channels in adult ventricular myocyte.

机构信息

Department of Cardiovascular Sciences, National Heart and Lung Institute, Imperial College London, UK.

The Leon H Charney Division of Cardiology, New York University School of Medicine, New York, NY, USA.

出版信息

Circ Res. 2013 Apr 12;112(8):1112-1120. doi: 10.1161/CIRCRESAHA.111.300445. Epub 2013 Feb 25.

Abstract

RATIONALE

Compartmentation of ion channels on the cardiomyocyte surface is important for electric propagation and electromechanical coupling. The specialized T-tubule and costameric structures facilitate spatial coupling of various ion channels and receptors. Existing methods such as immunofluorescence and patch clamp techniques are limited in their ability to localize functional ion channels. As such, a correlation between channel protein location and channel function remains incomplete.

OBJECTIVE

To validate a method that permits routine imaging of the topography of a live cardiomyocyte and study clustering of functional ion channels from a specific microdomain.

METHODS AND RESULTS

We used scanning ion conductance microscopy and conventional cell-attached patch clamp with a software modification that allows controlled increase of pipette tip diameter. The sharp nanopipette used for topography scan was modified into a larger patch pipette that could be positioned with nanoscale precision to a specific site of interest (crest, groove, or T-tubules of cardiomyocytes) and sealed to the membrane for cell-attached recording of ion channels. Using this method, we significantly increased the probability of detecting activity of L-type calcium channels in the T-tubules of ventricular cardiomyocytes. We also demonstrated that active sodium channels do not distribute homogenously on the sarcolemma instead, they segregate into clusters of various densities, most crowded in the crest region, that are surrounded by areas virtually free of functional sodium channels.

CONCLUSIONS

Our new method substantially increases the throughput of recording location-specific functional ion channels on the cardiomyocyte sarcolemma, thereby allowing characterization of ion channels in relation to the microdomain where they reside.

摘要

原理

心肌细胞表面离子通道的分隔对于电传播和机电耦联很重要。特化的 T 管和肌节结构有助于各种离子通道和受体的空间偶联。免疫荧光和膜片钳等现有方法在定位功能离子通道方面能力有限。因此,通道蛋白位置与通道功能之间的相关性仍不完整。

目的

验证一种常规成像活心肌细胞形貌并研究特定微域中功能性离子通道聚集的方法。

方法和结果

我们使用扫描离子电导显微镜和常规细胞贴附膜片钳,并进行软件修改,以允许控制吸管尖端直径的增加。用于形貌扫描的尖锐纳米吸管被修改为较大的贴片吸管,可以纳米级精度定位到感兴趣的特定部位(心室肌细胞的峰、谷或 T 管),并密封到细胞膜上,以进行细胞贴附离子通道记录。使用这种方法,我们显著增加了在心室肌细胞 T 管中检测 L 型钙通道活性的概率。我们还表明,活性钠通道不是均匀分布在肌节膜上,而是聚集在各种密度的簇中,在峰区最为拥挤,周围是几乎没有功能性钠通道的区域。

结论

我们的新方法大大提高了在心肌细胞膜上记录特定位置功能离子通道的通量,从而能够描述与它们所在微域相关的离子通道。

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