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豚鼠对咔哒声敏感的初级前庭传入神经的生理和解剖学研究。

Physiological and anatomical study of click-sensitive primary vestibular afferents in the guinea pig.

作者信息

Murofushi T, Curthoys I S

机构信息

Department of Psychology, University of Sydney, NSW, Australia.

出版信息

Acta Otolaryngol. 1997 Jan;117(1):66-72. doi: 10.3109/00016489709117994.

Abstract

We studied the sensitivity of primary vestibular afferents in anaesthetised guinea pigs to clicks. These vestibular neurons were also tested by their response to pitch and roll tilts and yaw-axis angular acceleration. The click intensity was referred to the threshold for evoking the auditory brainstem responses. Recording sites in the vestibular nerve were confirmed histologically using iontophoretic injection of FCF green dye. To confirm the site of labyrinthine origin of the click-sensitive neurons, we used retrograde tracing with biocytin. In all, 647 out of 2354 neurons in the vestibular nerves of 51 guinea pigs were activated by clicks. Most were irregularly discharging primary neurons, but some were regularly discharging. We studied responses to vestibular stimuli in 188 click-sensitive neurons. Of these, 86% responded to pitch and/or roll tilt, but none responded to yaw angular acceleration. Conversely we also recorded vestibular neurons which did not respond to clicks. None of 300 neurons sensitive to yaw angular acceleration were responsive to 80-90 dB SL clicks (0 dB SL = threshold for auditory brainstem response to clicks). The latencies of click-evoked action potentials of neurons in the vestibular nerve were very short (mean +/- SD = 0.82 +/- 0.22 ms). Changing click polarity caused a heterogeneous pattern of latency change. Thresholds for evoking spikes in primary vestibular neurons were high (62.0 +/- 12.2 dB SL, range 30-90 dB, n = 371). Retrograde tracing of the origin of the click-sensitive afferents using extracellular biocytin showed that most neurons originated in the medial (striola area) of the saccular macula.

摘要

我们研究了麻醉豚鼠初级前庭传入神经对咔嗒声的敏感性。这些前庭神经元还通过其对俯仰和横滚倾斜以及偏航轴角加速度的反应进行测试。咔嗒声强度以诱发听觉脑干反应的阈值为参考。使用离子电渗法注射FCF绿色染料,通过组织学方法确认前庭神经中的记录位点。为了确定对咔嗒声敏感神经元的迷路起源部位,我们使用生物素进行逆行追踪。在51只豚鼠的前庭神经中,2354个神经元中有647个被咔嗒声激活。大多数是不规则放电的初级神经元,但也有一些是规则放电的。我们研究了188个对咔嗒声敏感的神经元对前庭刺激的反应。其中,86%的神经元对俯仰和/或横滚倾斜有反应,但对偏航角加速度均无反应。相反我们还记录了对咔嗒声无反应的前庭神经元。300个对偏航角加速度敏感的神经元中,没有一个对80 - 90 dB SL的咔嗒声有反应(0 dB SL = 听觉脑干对咔嗒声反应的阈值)。前庭神经中神经元的咔嗒声诱发动作电位潜伏期非常短(平均值±标准差 = 0.82±0.22毫秒)。改变咔嗒声极性会导致潜伏期变化的异质性模式。在前庭初级神经元中诱发动作电位的阈值较高(62.0±12.2 dB SL,范围30 - 90 dB,n = 371)。使用细胞外生物素对咔嗒声敏感传入神经的起源进行逆行追踪显示,大多数神经元起源于球囊斑的内侧(纹区)。

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