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Kv1.3通道基因靶向缺失产生了具有改变的肾小球、相互作用的支架蛋白和生物物理学特性的“超级嗅觉小鼠”。

Kv1.3 channel gene-targeted deletion produces "Super-Smeller Mice" with altered glomeruli, interacting scaffolding proteins, and biophysics.

作者信息

Fadool D A, Tucker K, Perkins R, Fasciani G, Thompson R N, Parsons A D, Overton J M, Koni P A, Flavell R A, Kaczmarek L K

机构信息

Department of Biological Science, Programs in Neuroscience and Molecular Biophysics, The Florida State University, Tallahassee, FL 32306, USA.

出版信息

Neuron. 2004 Feb 5;41(3):389-404. doi: 10.1016/s0896-6273(03)00844-4.

Abstract

Mice with gene-targeted deletion of the Kv1.3 channel were generated to study its role in olfactory function. Potassium currents in olfactory bulb mitral cells from Kv1.3 null mice have slow inactivation kinetics, a modified voltage dependence, and a dampened C-type inactivation and fail to be modulated by activators of receptor tyrosine signaling cascades. Kv1.3 deletion increases expression of scaffolding proteins that normally regulate the channel through protein-protein interactions. Kv1.3-/- mice have a 1,000- to 10,000-fold lower threshold for detection of odors and an increased ability to discriminate between odorants. In accordance with this heightened sense of smell, Kv1.3-/- mice have glomeruli or olfactory coding units that are smaller and more numerous than those of wild-type mice. These data suggest that Kv1.3 plays a far more reaching role in signal transduction, development, and olfactory coding than that of the classically defined role of a potassium channel-to shape excitability by influencing membrane potential.

摘要

为了研究Kv1.3通道在嗅觉功能中的作用,构建了基因靶向缺失Kv1.3通道的小鼠。来自Kv1.3基因敲除小鼠嗅球二尖瓣细胞中的钾电流具有缓慢的失活动力学、改变的电压依赖性、减弱的C型失活,并且不能被受体酪氨酸信号级联反应的激活剂调节。Kv1.3的缺失增加了通常通过蛋白质-蛋白质相互作用调节该通道的支架蛋白的表达。Kv1.3基因敲除小鼠对气味检测的阈值降低了1000至10000倍,并且区分气味剂的能力增强。与这种增强的嗅觉一致,Kv1.3基因敲除小鼠的肾小球或嗅觉编码单元比野生型小鼠的更小且更多。这些数据表明,Kv1.3在信号转导、发育和嗅觉编码中所起的作用远比钾通道通过影响膜电位来塑造兴奋性这一经典定义的作用更为广泛。

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