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人类神经退行性疾病小鼠模型中姿势摆动的定量测量。

Quantitative measurement of postural sway in mouse models of human neurodegenerative disease.

作者信息

Hutchinson D, Ho V, Dodd M, Dawson H N, Zumwalt A C, Schmitt D, Colton C A

机构信息

Division of Neurology, Duke University Medical Center, Box 2900, Durham, NC 27710, USA.

出版信息

Neuroscience. 2007 Sep 21;148(4):825-32. doi: 10.1016/j.neuroscience.2007.07.025. Epub 2007 Jul 21.

Abstract

Detection of motor dysfunction in genetic mouse models of neurodegenerative disease requires reproducible, standardized and sensitive behavioral assays. We have utilized a center of pressure (CoP) assay in mice to quantify postural sway produced by genetic mutations that affect motor control centers of the brain. As a positive control for postural instability, wild type mice were injected with harmaline, a tremorigenic agent, and the average areas of the 95% confidence ellipse, which measures 95% of the CoP trajectory values recorded in a single trial, were measured. Ellipse area significantly increased in mice treated with increasing doses of harmaline and returned to control values after recovery. We also examined postural sway in mice expressing mutations that mimic frontotemporal dementia with Parkinsonism linked to chromosome 17 (FTDP-17) (T-279, P301L or P301L-nitric oxide synthase 2 (NOS2)(-/-) mice) and that demonstrate motor symptoms. These mice were then compared with a mouse model of Alzheimer's disease (APPSwDI mice) that demonstrates cognitive, but not motor deficits. T-279 and P301L-NOS2(-/-) mice demonstrated a significant increase in CoP ellipse area compared with appropriate wild type control mice or to mice expressing the P301L mutation alone. In contrast, postural instability was significantly reduced in APPSwDI mice that have cognitive deficits but do not have associated motor deficits. The CoP assay provides a simple, sensitive and quantitative tool to detect motor deficits resulting from postural abnormalities in mice and may be useful in understanding the underlying mechanisms of disease.

摘要

在神经退行性疾病的基因小鼠模型中检测运动功能障碍需要可重复、标准化且灵敏的行为学检测方法。我们利用小鼠的压力中心(CoP)检测方法来量化由影响大脑运动控制中心的基因突变所产生的姿势摆动。作为姿势不稳定的阳性对照,给野生型小鼠注射震颤剂哈马灵,并测量95%置信椭圆的平均面积,该椭圆测量的是单次试验中记录的CoP轨迹值的95%。用递增剂量哈马灵处理的小鼠中,椭圆面积显著增加,恢复后又回到对照值。我们还检测了表达模拟与17号染色体相关的帕金森病额颞叶痴呆(FTDP - 17)(T - 279、P301L或P301L - 一氧化氮合酶2(NOS2)敲除小鼠)且表现出运动症状的突变小鼠的姿势摆动。然后将这些小鼠与表现出认知缺陷但无运动缺陷的阿尔茨海默病小鼠模型(APPSwDI小鼠)进行比较。与相应的野生型对照小鼠或仅表达P301L突变的小鼠相比,T - 279和P301L - NOS2敲除小鼠的CoP椭圆面积显著增加。相比之下,有认知缺陷但无相关运动缺陷的APPSwDI小鼠的姿势不稳定显著降低。CoP检测提供了一种简单、灵敏且定量的工具,用于检测小鼠因姿势异常导致的运动缺陷,可能有助于理解疾病的潜在机制。

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