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Electrophysiological Assessment of Murine Atria with High-Resolution Optical Mapping

机译:高分辨率光学测绘对小鼠心房的电生理评估

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摘要

Recent genome-wide association studies targeting atrial fibrillation (AF) have indicated a strong association between the genotype and electrophysiological phenotype in the atria. That encourages us to utilize a genetically-engineered mouse model to elucidate the mechanism of AF. However, it is difficult to evaluate the electrophysiological properties in murine atria due to their small size. This protocol describes the electrophysiological evaluation of atria using an optical mapping system with a high temporal and spatial resolution in Langendorff perfused murine hearts. The optical mapping system is assembled with dual high-speed complementary metal oxide semiconductor cameras and high magnification objective lenses, to detect the fluorescence of a voltage-sensitive dye and Ca2+ indicator. To focus on the assessment of murine atria, optical mapping is performed with an area of 2 mm × 2 mm or 10 mm x 10 mm, with a 100 × 100 resolution (20 µm/pixel or 100 µm/pixel) and sampling rate of up to 10 kHz (0.1 ms) at maximum. A 1-French size quadripolar electrode pacing catheter is placed into the right atrium through the superior vena cava avoiding any mechanical damage to the atrium, and pacing stimulation is delivered through the catheter. An electrophysiological study is performed with programmed stimulation including constant pacing, burst pacing, and up to triple extrastimuli pacing. Under a spontaneous or pacing rhythm, the optical mapping recorded the action potential duration, activation map, conduction velocity, and Ca2+ transient individually in the right and left atria. In addition, the programmed stimulation also determines the inducibility of atrial tachyarrhythmias. Precise activation mapping is performed to identify the propagation of the excitation in the atrium during an induced atrial tachyarrhythmia. Optical mapping with a specialized setting enables a thorough electrophysiological evaluation of the atrium in murine pathological models.
机译:最近针对心房纤颤(AF)的全基因组关联研究表明,心房的基因型和电生理表型之间存在很强的关联。这鼓励我们利用基因工程小鼠模型阐明房颤的机制。然而,由于鼠心房的尺寸小,很难评估其电生理特性。该协议描述了在Langendorff灌注小鼠心脏中使用具有高时空分辨率的光学测绘系统对心房进行电生理评估的方法。该光学测绘系统由两个高速互补金属氧化物半导体照相机和高倍物镜组成,以检测电压敏感染料和Ca 2 + 指示剂的荧光。为了专注于评估鼠的心房,在2 mm×2 mm或10 mm x 10 mm的区域上以100×100的分辨率(20 µm /像素或100 µm /像素)进行光学映射,采样率为最高可达10 kHz(0.1 ms)。将1英寸大小的四极电极起搏导管通过上腔静脉放入右心房,避免对心房造成任何机械损伤,并且通过导管传递起搏刺激。用程序刺激进行电生理研究,包括持续起搏,突发起搏和多达三倍的额外刺激起搏。在自发或起搏节律下,光学测绘分别记录了左右心房中的动作电位持续时间,激活图,传导速度和Ca 2 + 瞬变。此外,程序性刺激还决定了房性快速性心律失常的可诱导性。进行精确的激活作图,以确定在诱发性房性心律失常期间心房中兴奋性的传播。具有特殊设置的光学标测可以在鼠类病理模型中对心房进行全面的电生理评估。

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