Single-cell brain atlas of Parkinson's disease mouse model

被引:0
作者
Jixing Zhong [1 ,2 ]
Gen Tang [3 ]
Jiacheng Zhu [2 ,4 ]
Weiying Wu [5 ]
Ge Li [6 ]
Xiumei Lin [2 ,4 ]
Langchao Liang [2 ,4 ]
Chaochao Chai [2 ,4 ]
Yuying Zeng [2 ,4 ]
Feiyue Wang [2 ,4 ]
Lihua Luo [2 ,4 ]
Jiankang Li [2 ]
Fang Chen [2 ,7 ]
Zhen Huang [8 ,9 ]
Xiuqing Zhang [2 ]
Yu Zhang [6 ]
Hongde Liu [1 ]
Xin Qiu [3 ]
Shengping Tang [3 ]
Dongsheng Chen [2 ]
机构
[1] School of Biological Science & Medical Engineering, Southeast University
[2] BGI-Shenzhen
[3] Shenzhen Children's Hospital
[4] BGI Education Center, University of Chinese Academy of Sciences
[5] Department of Neurobiology, NHC and CAMS Key Laboratory of Medical Neurobiology, School of Brain Science and Brian Medicine, And the MOE Frontier Science Center for Brain Research and Brain-Machine Integration, Zhejiang University School of Medicine 
[6] MGI,BGI-Shenzhen
[7] Life Science College, Fujian Normal University
[8] Key Laboratory of Special Marine Bio-resources Sustainable Utilization of Fujian Province
基金
中国国家自然科学基金;
关键词
D O I
暂无
中图分类号
R742.5 [震颤麻痹综合征];
学科分类号
1002 ;
摘要
Parkinson’s disease(PD) is a neurodegenerative disease, leading to the impairment of movement execution. PD pathogenesis has been largely investigated, either limited to bulk transcriptomic levels or at certain cell types, which failed to capture the cellular heterogeneity and intrinsic interplays among distinct cell types. Here, we report the application of single-nucleus RNA-seq on midbrain, striatum, and cerebellum of the α-syn-A53 T mouse, a well-established PD mouse model, and matched controls, generating the first single cell transcriptomic atlas for the PD model mouse brain composed of 46,174 individual cells. Additionally, we comprehensively depicte the dysfunctions in PD pathology, covering the elevation of NF-k B activity, the alteration of ion channel components, the perturbation of protein homeostasis network, and the dysregulation of glutamatergic signaling. Notably, we identify a variety of cell types closely associated with PD risk genes. Taken together, our study provides valuable resources to systematically dissect the molecular mechanism of PD pathogenesis at the single-cell resolution, which facilitates the development of novel approaches for diagnosis and therapies against PD.
引用
收藏
页码:277 / 288
页数:12
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