首页> 美国卫生研究院文献>The Journal of Neuroscience >Nanoscale Organization of the MEC-4 DEG/ENaC Sensory Mechanotransduction Channel in Caenorhabditis elegans Touch Receptor Neurons
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Nanoscale Organization of the MEC-4 DEG/ENaC Sensory Mechanotransduction Channel in Caenorhabditis elegans Touch Receptor Neurons

机译:秀丽隐杆线虫触摸受体神经元中MEC-4 DEG / ENaC感觉机械传递通道的纳米级组织。

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摘要

Hearing, touch and proprioception are thought to involve direct activation of mechano-electrical transduction (MeT) channels. In Caenorhabditis elegans touch receptor neurons (TRNs), such channels contain two pore-forming subunits (MEC-4 and MEC-10) and two auxiliary subunits (MEC-2 and MEC-6). MEC-4 and MEC-10 belong to a large superfamily of ion channel proteins (DEG/ENaCs) that form nonvoltage-gated, amiloride-sensitive Na+ channels. In TRNs, unique 15-protofilament microtubules and an electron-dense extracellular matrix have been proposed to serve as gating tethers critical for MeT channel activation. We combined high-pressure freezing and serial-section immunoelectron microscopy to determine the position of MeT channels relative to putative gating tethers. MeT channels were visualized using antibodies against MEC-4 and MEC-2. This nanometer-resolution view of a sensory MeT channel establishes structural constraints on the mechanics of channel gating. We show here that MEC-2 and MEC-5 collagen, a putative extracellular tether, occupy overlapping but distinct domains in TRN neurites. Although channels decorate all sides of TRN neurites; they are not associated with the distal endpoints of 15-protofilament microtubules hypothesized to be gating tethers. These specialized microtubules, which are unique to TRNs, assemble into a cross-linked bundle connected by a network of kinked filaments to the neurite membrane. We speculate that the microtubule bundle converts external point loads into membrane stretch which, in turn, facilitates MeT channel activation.
机译:听力,触觉和本体感觉被认为涉及直接的机电转换(MeT)通道激活。在秀丽隐杆线虫触摸受体神经元(TRN)中,此类通道包含两个成孔亚基(MEC-4和MEC-10)和两个辅助亚基(MEC-2和MEC-6)。 MEC-4和MEC-10属于离子通道蛋白(DEG / ENaCs)的超家族,可形成非电压门控,阿米洛利敏感的Na + 通道。在TRNs中,已经提出了独特的15条原丝微管和一种电子致密的细胞外基质,作为对MeT通道激活至关重要的门控系链。我们结合高压冷冻和连续切片免疫电子显微镜来确定MeT通道相对于假定的门控系链的位置。使用针对MEC-4和MEC-2的抗体可视化MeT通道。感官MeT通道的这种纳米分辨率视图对通道门控的力学建立了结构约束。我们在这里显示,MEC-2和MEC-5胶原蛋白(一种推测的细胞外系链)在TRN神经突中占据重叠但截然不同的域。尽管通道装饰着TRN神经突的所有侧面;它们与假设为门控系链的15条原丝微管的远端端点无关。这些专门的微管是TRN所特有的,它们组装成交联的束,通过扭结的细丝网络连接到神经突膜上。我们推测,微管束将外部点载荷转换为膜拉伸,从而促进MeT通道激活。

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