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本文引用的文献

1
Preparation of gene gun bullets and biolistic transfection of neurons in slice culture.基因枪子弹的制备及脑片培养中神经元的生物弹道转染
J Vis Exp. 2008 Feb 13(12):675. doi: 10.3791/675.
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A method for chronic stimulation of cortical organotypic cultures using implanted electrodes.一种使用植入电极对皮质器官型培养物进行慢性刺激的方法。
J Neurosci Methods. 2009 Jan 30;176(2):136-43. doi: 10.1016/j.jneumeth.2008.08.037. Epub 2008 Sep 13.
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Gene-gun transfection of hippocampal neurons.海马神经元的基因枪转染
J Vis Exp. 2006 Nov 30(1):121. doi: 10.3791/121.
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Preparation and maintenance of organotypic slice cultures of CNS tissue.中枢神经系统组织器官型切片培养物的制备与维持
Curr Protoc Neurosci. 2001 May;Chapter 6:Unit 6.11. doi: 10.1002/0471142301.ns0611s09.
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Development and plasticity of spontaneous activity and Up states in cortical organotypic slices.皮质器官型切片中自发活动和去极化状态的发育与可塑性
J Neurosci. 2007 May 30;27(22):5915-25. doi: 10.1523/JNEUROSCI.0447-07.2007.
6
Mechanism of the 5-hydroxytryptamine 2A receptor-mediated facilitation of synaptic activity in prefrontal cortex.5-羟色胺2A受体介导的前额叶皮质突触活动促进机制
Proc Natl Acad Sci U S A. 2007 Jun 5;104(23):9870-5. doi: 10.1073/pnas.0700436104. Epub 2007 May 29.
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Biolistic transfection of neuronal cultures using a hand-held gene gun.使用手持式基因枪对神经元培养物进行生物弹道转染。
Nat Protoc. 2006;1(2):977-81. doi: 10.1038/nprot.2006.145.
8
Kv2 subunits underlie slowly inactivating potassium current in rat neocortical pyramidal neurons.Kv2亚基是大鼠新皮层锥体神经元中缓慢失活钾电流的基础。
J Physiol. 2007 Jun 15;581(Pt 3):941-60. doi: 10.1113/jphysiol.2007.128454. Epub 2007 Mar 22.
9
Functional roles of Kv1 channels in neocortical pyramidal neurons.Kv1通道在新皮质锥体神经元中的功能作用。
J Neurophysiol. 2007 Mar;97(3):1931-40. doi: 10.1152/jn.00933.2006. Epub 2007 Jan 10.
10
Expression and biophysical properties of Kv1 channels in supragranular neocortical pyramidal neurones.颗粒上层新皮质锥体神经元中Kv1通道的表达及生物物理特性
J Physiol. 2006 Mar 1;571(Pt 2):371-89. doi: 10.1113/jphysiol.2005.097006. Epub 2005 Dec 22.

来自新皮质器官型切片标本的全细胞记录。

Whole cell recording from an organotypic slice preparation of neocortex.

作者信息

Foehring Robert C, Guan Dongxu, Toleman Tara, Cantrell Angela R

机构信息

Department of Anatomy and Neurobiology, University of Tennessee Health Science Center, USA.

出版信息

J Vis Exp. 2011 Jun 3(52):2600. doi: 10.3791/2600.

DOI:10.3791/2600
PMID:21673642
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3197031/
Abstract

We have been studying the expression and functional roles of voltage-gated potassium channels in pyramidal neurons from rat neocortex. Because of the lack of specific pharmacological agents for these channels, we have taken a genetic approach to manipulating channel expression. We use an organotypic culture preparation (16) in order to maintain cell morphology and the laminar pattern of cortex. We typically isolate acute neocortical slices at postnatal days 8-10 and maintain the slices in culture for 3-7 days. This allows us to study neurons at a similar age to those in our work with acute slices and minimizes the development of exuberant excitatory connections in the slice. We record from visually-identified pyramidal neurons in layers II/III or V using infrared illumination (IR-) and differential interference contrast microscopy (DIC) with whole cell patch clamp in current- or voltage-clamp. We use biolistic (Gene gun) transfection of wild type or mutant potassium channel DNA to manipulate expression of the channels to study their function. The transfected cells are easily identified by epifluorescence microscopy after co-transfection with cDNA for green fluorescent protein (GFP). We compare recordings of transfected cells to adjacent, untransfected neurons in the same layer from the same slice.

摘要

我们一直在研究电压门控钾通道在大鼠新皮质锥体神经元中的表达及功能作用。由于缺乏针对这些通道的特异性药理试剂,我们采用了基因方法来操纵通道表达。我们使用器官型培养制剂(16)以维持细胞形态和皮质的层状模式。我们通常在出生后第8 - 10天分离急性新皮质切片,并将切片在培养中维持3 - 7天。这使我们能够研究与我们在急性切片实验中处于相似年龄的神经元,并最大限度地减少切片中过度兴奋性连接的形成。我们使用红外照明(IR -)和微分干涉对比显微镜(DIC),通过全细胞膜片钳在电流钳或电压钳模式下,从视觉识别的II/III层或V层锥体神经元进行记录。我们使用生物弹道式(基因枪)转染野生型或突变型钾通道DNA来操纵通道表达,以研究其功能。在与绿色荧光蛋白(GFP)的cDNA共转染后,通过落射荧光显微镜很容易识别转染的细胞。我们将转染细胞的记录与来自同一切片同一层中相邻的未转染神经元的记录进行比较。