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基于延迟线反符合探测的亚毫秒级尖峰时间差异检测。

Detection of submillisecond spike timing differences based on delay-line anticoincidence detection.

机构信息

Department of Biology, Washington University in St. Louis, St. Louis, Missouri;

出版信息

J Neurophysiol. 2013 Nov;110(10):2295-311. doi: 10.1152/jn.00444.2013. Epub 2013 Aug 21.

Abstract

Detection of submillisecond interaural timing differences is the basis for sound localization in reptiles, birds, and mammals. Although comparative studies reveal that different neural circuits underlie this ability, they also highlight common solutions to an inherent challenge: processing information on timescales shorter than an action potential. Discrimination of small timing differences is also important for species recognition during communication among mormyrid electric fishes. These fishes generate a species-specific electric organ discharge (EOD) that is encoded into submillisecond-to-millisecond timing differences between receptors. Small, adendritic neurons (small cells) in the midbrain are thought to analyze EOD waveform by comparing these differences in spike timing, but direct recordings from small cells have been technically challenging. In the present study we use a fluorescent labeling technique to obtain visually guided extracellular recordings from individual small cell axons. We demonstrate that small cells receive 1-2 excitatory inputs from 1 or more receptive fields with latencies that vary by over 10 ms. This wide range of excitatory latencies is likely due to axonal delay lines, as suggested by a previous anatomic study. We also show that inhibition of small cells from a calyx synapse shapes stimulus responses in two ways: through tonic inhibition that reduces spontaneous activity and through precisely timed, stimulus-driven, feed-forward inhibition. Our results reveal a novel delay-line anticoincidence detection mechanism for processing submillisecond timing differences, in which excitatory delay lines and precisely timed inhibition convert a temporal code into a population code.

摘要

检测亚毫秒级的耳间时间差异是爬行动物、鸟类和哺乳动物进行声音定位的基础。尽管比较研究揭示了不同的神经回路是这种能力的基础,但它们也突出了应对固有挑战的共同解决方案:即在动作电位时间尺度更短的情况下处理信息。在电鳗鱼类的通讯中,对小时间差异的辨别对于物种识别也很重要。这些鱼类产生特定于物种的电器官放电 (EOD),这些放电以受体之间的亚毫秒到毫秒时间差异进行编码。中脑的小型无树突神经元(小细胞)被认为通过比较这些尖峰时间差异来分析 EOD 波形,但从小细胞进行直接记录在技术上具有挑战性。在本研究中,我们使用荧光标记技术从单个小细胞轴突获得视觉引导的细胞外记录。我们证明小细胞从 1 个或多个感受野接收 1-2 个兴奋性输入,其潜伏期相差超过 10 毫秒。这种广泛的兴奋性潜伏期可能是由于轴突延迟线所致,正如先前的解剖学研究所示。我们还表明,来自耳石突触的小细胞抑制以两种方式塑造刺激反应:通过减少自发活动的紧张性抑制,以及通过精确计时、刺激驱动的前馈抑制。我们的研究结果揭示了一种用于处理亚毫秒级时间差异的新型延迟线符合检测机制,其中兴奋性延迟线和精确计时的抑制将时间编码转换为群体编码。

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本文引用的文献

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The calyx of Held synapse: from model synapse to auditory relay.Held 突触花萼:从模式突触到听觉中继。
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