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精神分裂症患者背外侧前额叶皮质中小白蛋白篮状细胞输入的改变。

Altered parvalbumin basket cell inputs in the dorsolateral prefrontal cortex of schizophrenia subjects.

作者信息

Glausier J R, Fish K N, Lewis D A

机构信息

Department of Psychiatry, University of Pittsburgh School of Medicine, Pittsburgh, PA, USA.

Department of Neuroscience, University of Pittsburgh, Pittsburgh, PA, USA.

出版信息

Mol Psychiatry. 2014 Jan;19(1):30-6. doi: 10.1038/mp.2013.152. Epub 2013 Nov 12.

DOI:10.1038/mp.2013.152
PMID:24217255
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3874728/
Abstract

Cortical circuitry dysfunction in schizophrenia has been studied at many different levels of resolution, but not at the most basic unit of network organization--synaptic inputs. Multi-label electron or confocal light microscopy is required to examine specific types of synaptic inputs, and application of these methods to quantitatively study disease-related changes in human postmortem tissue has not been feasible for technical reasons. We recently developed a multi-label confocal light microscopic approach that makes possible the systematic identification and quantification of synaptic inputs, and of the relative levels of proteins localized to these inputs, in human postmortem tissue. We applied this approach to quantify parvalbumin basket cell (PVBC) inputs in area 9 of the dorsolateral prefrontal cortex from schizophrenia and matched comparison subjects. Tissue sections were triple-labeled for the 65 kD isoform of glutamic acid decarboxylase (GAD65), PV and the GABA(A) receptor α1 subunit. PVBC axonal boutons were defined as PV/GAD65 dual-labeled puncta, and PVBC inputs were defined as a PVBC bouton that overlapped a GABA(A) receptor α1 subunit punctum. The density of PVBC inputs was unchanged in subjects with schizophrenia, but levels of PV protein were lower in PVBC boutons. In concert with prior reports, these findings indicate that PVBC dysfunction in schizophrenia reflects molecular and not structural alterations in these cells and their axon terminals.

摘要

精神分裂症中皮质神经回路功能障碍已在许多不同分辨率水平上进行了研究,但尚未在网络组织的最基本单位——突触输入层面进行研究。需要多标记电子显微镜或共聚焦光学显微镜来检查特定类型的突触输入,由于技术原因,将这些方法应用于定量研究人类死后组织中与疾病相关的变化并不可行。我们最近开发了一种多标记共聚焦光学显微镜方法,使得在人类死后组织中系统地识别和定量突触输入以及定位于这些输入的蛋白质的相对水平成为可能。我们应用这种方法对精神分裂症患者和匹配的对照受试者背外侧前额叶皮质9区的小白蛋白篮状细胞(PVBC)输入进行定量。组织切片用谷氨酸脱羧酶65kD亚型(GAD65)、小白蛋白(PV)和γ-氨基丁酸A型受体α1亚基进行三重标记。PVBC轴突终扣被定义为PV/GAD65双标记的小点,PVBC输入被定义为与γ-氨基丁酸A型受体α1亚基小点重叠的PVBC终扣。精神分裂症患者的PVBC输入密度没有变化,但PVBC终扣中的PV蛋白水平较低。与先前的报道一致,这些发现表明精神分裂症中PVBC功能障碍反映了这些细胞及其轴突终末的分子而非结构改变。

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