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Electrophysiological properties of lumbosacral primary afferent neurons innervating urothelial and non-urothelial layers of mouse urinary bladder

机译:腰s神经支配小鼠膀胱尿路上皮层和非尿路上皮层的电生理特性

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摘要

Pelvic nerve (PN) bladder primary afferent neurons were retrogradely labeled by intraparenchymal (IPar) microinjection of fluorescent tracer or intravesical (IVes) infusion of tracer into the bladder lumen. IPar and IVes techniques labeled two distinct populations of PN bladder neurons differentiated on the basis of dorsal root ganglion (DRG) soma labeling, dye distribution within the bladder, and intrinsic electrophysiological properties. IPar (Fast blue)- and IVes (DiI)-labeled neurons accounted for 91.5% (378.3 ± 32.3) and 8% (33.0 ± 26.0) of all labeled neurons, respectively (p<0.01), with only 2.0 ± 1.2 neurons labeled by both techniques. When dyes were switched, IPar (DiI)- and IVes (Fast blue) labeled neurons accounted for 77.6% (103.0 ± 25.8) and 22.4% (29.8 ± 10.5), respectively (P<0.05), with 6.0 ± 1.5 double-labeled neurons. Following IPar labeling, DiI was distributed throughout non-urothelial layers of the bladder. In contrast, dye was contained within the urothelium and occasionally the submucosa after IVes labeling. Electrophysiological properties of DiI-labeled IPar and IVes DRG neurons were characterized by whole-mount, in situ patch-clamp recordings. IPar- and IVes-labeled neurons differed significantly with respect to rheobase, input resistance, membrane capacitance, amplitude of inactivating and sustained K+ currents, and rebound action potential firing, suggesting that the IVes population is more excitable. This study is the first to demonstrate that IVes labeling is a minimally invasive approach for retrograde labeling of PN bladder afferent neurons, to selectively identify urothelial versus non-urothelial bladder DRG neurons, and to elucidate electrophysiological properties of urothelial and non-urothelial afferents in an intact DRG soma preparation.
机译:盆腔神经(PN)膀胱原发性传入神经元通过实质性内(IPar)荧光示踪剂显微注射或膀胱内(IVes)示踪剂注入膀胱内腔进行逆行标记。 IPar和IVes技术标记了两个不同的PN膀胱神经元群体,这些群体是根据背根神经节(DRG)躯体标记,膀胱内的染料分布以及固有的电生理特性而区分的。 IPar(深蓝色)和IVes(DiI)标记的神经元分别占所有标记神经元的91.5%(378.3±32.3)和8%(33.0±26.0),仅标记了2.0±1.2神经元通过两种技术。更换染料时,IPar(DiI)-和IVes(快速蓝)标记的神经元分别占77.6%(103.0±25.8)和22.4%(29.8±10.5)(P <0.05),其中有6.0±1.5双标记神经元。 IPar标记后,DiI分布在膀胱的非尿路上皮层。相反,在IVes标记后,染料被包含在尿路上皮中,偶尔包含在粘膜下层。 DiI标记的IPar和IVes DRG神经元的电生理特性通过完整的原位膜片钳记录来表征。 IPar和IVes标记的神经元在流变碱,输入电阻,膜电容,失活和持续K + 电流的幅度以及回弹动作电位触发方面有显着差异,这表明IVes种群更易激发。这项研究首次证明IVes标记是一种微创方法,用于对PN膀胱传入神经元进行逆向标记,选择性识别尿路上皮与非尿路上皮DRG神经元,并阐明尿路上皮和非尿路上皮传入神经的电生理特性。完整的DRG躯体准备。

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