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使用笼锁型谷氨酸进行光刺激揭示了活脑切片中的功能电路。

Photostimulation using caged glutamate reveals functional circuitry in living brain slices.

作者信息

Callaway E M, Katz L C

机构信息

Department of Neurobiology, Duke University Medical Center, Durham, NC 27710.

出版信息

Proc Natl Acad Sci U S A. 1993 Aug 15;90(16):7661-5. doi: 10.1073/pnas.90.16.7661.

DOI:10.1073/pnas.90.16.7661
PMID:7689225
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC47202/
Abstract

An approach for high-spatial-resolution mapping of functional circuitry in living mammalian brain slices has been developed. The locations of neurons making functional synaptic connections to a single neuron are revealed by photostimulation of highly restricted areas of the slice (50-100 microns in diameter) while maintaining a whole-cell recording of the neuron of interest. Photostimulation is achieved by bathing brain slices in a molecularly caged form of the neurotransmitter glutamate [L-glutamic acid alpha-(4,5-dimethoxy-2-nitrobenzyl) ester], which is then converted to the active form by brief pulses (< 1 ms in duration) of ultraviolet irradiation. Direct activation of receptors on recorded neurons in rat hippocampus and ferret visual cortex demonstrates that photostimulation is reliable and reproducible and can be repeated at the same site at least 30 times without obvious decrement in neuronal responsiveness. Photostimulation of presynaptic neurons at sites distant to the recorded neuron evoked synaptic responses in hippocampal and cortical cells at distances of up to several millimeters from the recorded neuron. Stimulation of 25-100 distinct presynaptic sites while recording from a single postsynaptic neuron was easily achieved. Caged glutamate-based photostimulation eliminates artifacts and limitations inherent in conventional stimulation methods, including stimulation of axons of passage, desensitization, and poor temporal resolution of "puffer" pipettes, and current artifacts of iontophoretic application. This approach allows detailed physiological investigation and manipulation of the complex intrinsic circuitry of the mammalian brain.

摘要

一种用于对活体哺乳动物脑切片中的功能回路进行高空间分辨率映射的方法已被开发出来。通过对切片的高度受限区域(直径50 - 100微米)进行光刺激,同时对感兴趣的神经元进行全细胞记录,来揭示与单个神经元形成功能性突触连接的神经元的位置。光刺激是通过将脑切片浸泡在神经递质谷氨酸的分子笼形式[L - 谷氨酸α - (4,5 - 二甲氧基 - 2 - 硝基苄基)酯]中来实现的,然后通过短暂的紫外线照射脉冲(持续时间<1毫秒)将其转化为活性形式。对大鼠海马体和雪貂视觉皮层中记录的神经元上的受体进行直接激活表明,光刺激是可靠且可重复的,并且可以在同一位点重复至少30次而神经元反应性无明显下降。在距记录神经元数毫米远的位点对突触前神经元进行光刺激,可在海马体和皮层细胞中诱发突触反应。从单个突触后神经元进行记录时,轻松实现对25 - 100个不同突触前位点的刺激。基于分子笼谷氨酸的光刺激消除了传统刺激方法固有的伪迹和局限性,包括对过路轴突的刺激、脱敏以及“吹管”移液管的时间分辨率差,以及离子电渗应用的电流伪迹。这种方法允许对哺乳动物脑的复杂内在回路进行详细的生理研究和操纵。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3bd0/47202/d31623a860f5/pnas01473-0249-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3bd0/47202/6c1aabfb2b64/pnas01473-0248-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3bd0/47202/d31623a860f5/pnas01473-0249-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3bd0/47202/6c1aabfb2b64/pnas01473-0248-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3bd0/47202/d31623a860f5/pnas01473-0249-a.jpg

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