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当前使用电压成像记录快速神经元活动的实践:无脊椎动物到哺乳动物研究中的成功案例。

Current Practice in Using Voltage Imaging to Record Fast Neuronal Activity: Successful Examples from Invertebrate to Mammalian Studies.

机构信息

Institute of Higher Nervous Activity and Neurophysiology, Russian Academy of Sciences, Butlerova 5A, Moscow 117485, Russia.

出版信息

Biosensors (Basel). 2023 Jun 13;13(6):648. doi: 10.3390/bios13060648.


DOI:10.3390/bios13060648
PMID:37367013
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10296598/
Abstract

The optical imaging of neuronal activity with potentiometric probes has been credited with being able to address key questions in neuroscience via the simultaneous recording of many neurons. This technique, which was pioneered 50 years ago, has allowed researchers to study the dynamics of neural activity, from tiny subthreshold synaptic events in the axon and dendrites at the subcellular level to the fluctuation of field potentials and how they spread across large areas of the brain. Initially, synthetic voltage-sensitive dyes (VSDs) were applied directly to brain tissue via staining, but recent advances in transgenic methods now allow the expression of genetically encoded voltage indicators (GEVIs), specifically in selected neuron types. However, voltage imaging is technically difficult and limited by several methodological constraints that determine its applicability in a given type of experiment. The prevalence of this method is far from being comparable to patch clamp voltage recording or similar routine methods in neuroscience research. There are more than twice as many studies on VSDs as there are on GEVIs. As can be seen from the majority of the papers, most of them are either methodological ones or reviews. However, potentiometric imaging is able to address key questions in neuroscience by recording most or many neurons simultaneously, thus providing unique information that cannot be obtained via other methods. Different types of optical voltage indicators have their advantages and limitations, which we focus on in detail. Here, we summarize the experience of the scientific community in the application of voltage imaging and try to evaluate the contribution of this method to neuroscience research.

摘要

通过同时记录多个神经元,电位探针的神经元活动光学成像技术已被认为能够解决神经科学中的关键问题。该技术由 50 年前首创,使研究人员能够研究神经活动的动态,从轴突和树突中微小的亚阈突触事件到场电位的波动以及它们如何在大脑的大片区域中传播。最初,通过染色将合成电压敏感染料(VSD)直接应用于脑组织,但目前在转基因方法方面的进展现在允许表达基因编码的电压指示剂(GEVI),特别是在选定的神经元类型中。然而,电压成像技术具有一定的难度,受到多种方法学限制的限制,这些限制决定了其在特定实验类型中的适用性。这种方法的普及程度远不能与膜片钳电压记录或神经科学研究中的类似常规方法相媲美。VSD 的研究比 GEVIs 多两倍以上。从大多数论文中可以看出,其中大多数是方法学论文或综述。然而,通过同时记录大多数或许多神经元,电位成像能够解决神经科学中的关键问题,从而提供无法通过其他方法获得的独特信息。不同类型的光学电压指示剂具有其优势和局限性,我们将对此进行详细讨论。在这里,我们总结了科学界在电压成像应用方面的经验,并尝试评估该方法对神经科学研究的贡献。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/08f9d96aa6b1/biosensors-13-00648-g004.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/a57f56dc1035/biosensors-13-00648-g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/0fc7b1045e7a/biosensors-13-00648-g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/f8d49280ccf6/biosensors-13-00648-g003.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/08f9d96aa6b1/biosensors-13-00648-g004.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/a57f56dc1035/biosensors-13-00648-g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/0fc7b1045e7a/biosensors-13-00648-g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/f8d49280ccf6/biosensors-13-00648-g003.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dbb2/10296598/08f9d96aa6b1/biosensors-13-00648-g004.jpg

相似文献

[1]
Current Practice in Using Voltage Imaging to Record Fast Neuronal Activity: Successful Examples from Invertebrate to Mammalian Studies.

Biosensors (Basel). 2023-6-13

[2]
In Vivo Observations of Rapid Scattered Light Changes Associated with Neurophysiological Activity

2009

[3]
Genetically Encoded Voltage Indicators: Opportunities and Challenges.

J Neurosci. 2016-9-28

[4]
In vivo wide-field voltage imaging in zebrafish with voltage-sensitive dye and genetically encoded voltage indicator.

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[5]
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[6]
Imaging different cell populations in the mouse olfactory bulb using the genetically encoded voltage indicator ArcLight.

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[7]
Current progress in genetically encoded voltage indicators for neural activity recording.

Curr Opin Chem Biol. 2016-8

[8]
Studying Synaptically Evoked Cortical Responses With Combination of a Single Neuron Recording (Whole-Cell) and Population Voltage Imaging (Genetically Encoded Voltage Indicator).

Front Neurosci. 2021-10-27

[9]
Comparative performance of a genetically-encoded voltage indicator and a blue voltage sensitive dye for large scale cortical voltage imaging.

Front Cell Neurosci. 2015-4-24

[10]
Toward Better Genetically Encoded Sensors of Membrane Potential.

Trends Neurosci. 2016-5

引用本文的文献

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Front Neurosci. 2025-1-8

[2]
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[3]
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本文引用的文献

[1]
Video-based pooled screening yields improved far-red genetically encoded voltage indicators.

Nat Methods. 2023-7

[2]
Dual-polarity voltage imaging of the concurrent dynamics of multiple neuron types.

Science. 2022-11-4

[3]
On the fluorescence enhancement of arch neuronal optogenetic reporters.

Nat Commun. 2022-10-28

[4]
Microstimulation in the primary visual cortex: activity patterns and their relation to visual responses and evoked saccades.

Cereb Cortex. 2023-4-25

[5]
Sustained deep-tissue voltage recording using a fast indicator evolved for two-photon microscopy.

Cell. 2022-9-1

[6]
A CCR5 antagonist, maraviroc, alleviates neural circuit dysfunction and behavioral disorders induced by prenatal valproate exposure.

J Neuroinflammation. 2022-7-29

[7]
Evoked Cortical Depolarizations Before and After the Amyloid Plaque Accumulation: Voltage Imaging Study.

J Alzheimers Dis. 2022

[8]
Thalamic bursting and the role of timing and synchrony in thalamocortical signaling in the awake mouse.

Neuron. 2022-9-7

[9]
Conserved Amino Acids Residing Outside the Voltage Field Can Shift the Voltage Sensitivity and Increase the Signal Speed and Size of Based GEVIs.

Front Cell Dev Biol. 2022-6-16

[10]
Differences in action potential propagation speed and axon initial segment plasticity between neurons from Sprague-Dawley rats and C57BL/6 mice.

Zool Res. 2022-7-18

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