Odour-evoked [Ca2+] transients in mitral cell dendrites of frog olfactory glomeruli.

K. Delaney, I. Davison, W. Denk
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引用次数: 23

Abstract

We measured Ca2+ concentration, [Ca2+], transients in mitral cell distal apical dendritic tufts produced by physiological odour stimulation of the olfactory epithelium and electrical stimulation of the olfactory nerve (ON) using two-photon scanning and conventional wide-field microscopy of Ca2+-Green-1 dextran in an in vitro frog nose-brain preparation. Weak or strong ON shock-evoked fluorescence transients always had short latency with an onset 0-10 ms after the onset of the bulb local field potential, rapidly increasing to a peak of up to 25% fractional fluorescence change (DeltaF/F) in 10-30 ms, were blocked by 10 microM CNQX, decaying with a time constant of about 1 s. With stronger ON shocks that activated many receptor axons, an additional, delayed, sustained AP5-sensitive component (peak at approximately 0.5 s, up to 40% DeltaF/F maximum) could usually be produced. Odour-evoked [Ca2+] transients sometimes displayed a rapid onset phase that peaked within 50 ms but always had a sustained phase that peaked 0.5-1.5 s after onset, regardless of the strength of the odour or the amplitude of the response. These were considerably larger (up to 150% DeltaF/F) than those evoked by ON shock. Odour-evoked [Ca2+] transients were also distinguished from ON shock-evoked transients by tufts in different glomeruli responding with different delays (time to onset differed by up to 1.5 s between different tufts for the same odour). Odour-evoked [Ca2+] transients were increased by AMPA-kainate receptor blockade, but substantially blocked by AP5. Electrical stimulation of the lateral olfactory tract (5-6 stimuli at 10 Hz) that evoked granule cell feedback inhibition, blocked 60-100% of the odour-evoked [Ca2+] transient in tufts when delivered within about 0.5 s of the odour. LOT-mediated inhibition was blocked by 10 microM bicuculline.
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气味诱发的蛙嗅肾小球二尖瓣细胞树突[Ca2+]瞬变。
我们测量了Ca2+浓度,[Ca2+],在二尖瓣细胞远端树突丛的瞬态产生的嗅觉上皮的生理气味刺激和嗅觉神经(ON)的电刺激,使用双光子扫描和常规宽视场显微镜Ca2+-Green-1葡聚糖在离体青蛙鼻脑制备。弱或强ON冲击诱发的荧光瞬态总是具有较短的潜伏期,在鳞茎局部场电位开始后0-10 ms开始,在10-30 ms内迅速增加到高达25%分数荧光变化(DeltaF/F)的峰值,被10微米的CNQX阻断,以约1 s的时间常数衰减。当更强的ON冲击激活许多受体轴突时,通常会产生额外的、延迟的、持续的ap5敏感成分(峰值约为0.5 s,最高可达40% δ F/F)。气味诱发的[Ca2+]瞬态有时表现为快速发作阶段,在50 ms内达到峰值,但无论气味强度或反应幅度如何,总是在发作后0.5-1.5 s达到峰值的持续阶段。这些比ON电击引起的大得多(高达150% δ F/F)。气味诱发的[Ca2+]瞬变也可以通过不同肾小球的簇状体以不同的延迟反应来区别于ON休克诱发的瞬变(对于相同的气味,不同簇状体的起效时间差异可达1.5 s)。气味诱发的[Ca2+]瞬态通过AMPA-kainate受体阻断而增加,但被AP5大量阻断。侧嗅道的电刺激(5-6次10赫兹的刺激)引起颗粒细胞反馈抑制,在气味大约0.5秒内传递时,阻断了60-100%的气味诱发的[Ca2+]瞬态。10微米二球茎碱阻断lot介导的抑制作用。
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