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Assessment of DNA replication in central nervous system by Laser Scanning Cytometry

机译:激光扫描细胞术评估中枢神经系统中的DNA复制

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In neurons of patients with Alzheimer's disease (AD) signs of cell cycle re-entry as well as polyploidy have been reported, indicating that the entire or a part of the genome of the neurons is duplicated before its death but mitosis is not initiated so that the cellular DNA content remains tetraploid. It was concluded, that this imbalance is the direct cause of the neuronal loss in AD. Manual counting of polyploidal cells is possible but time consuming and possibly statistically insufficient. The aim of this study was to develop an automated method that detects the neuronal DNA content abnormalities with Laser Scanning Cytometry (LSC).Frozen sections of formalin-fixed brain tissue of AD patients and control subjects were labelled with anti-cyclin B and anti-NeuN antibodies. Immunolabelling was performed using Cy5- and Cy2-conjugated secondary antibodies and biotin streptavidin or tyramid signal amplification. In the end sections of 20 μm thickness were incubated with propidium iodide (PI) (50μg/ml) and covered on slides. For analysis by the LSC PI was used as trigger. Cells identified as neurons by NeuN expression were analyzed for cyclin B expression. Per specimen data of at least 10,000 neurons were acquired. In the frozen brain sections an automated quantification of the amount of nuclear DNA is possible with LSC. The DNA ploidy as well as the cell cycle distribution can be analyzed. A high number of neurons can be scanned and the duration of measuring is shorter than a manual examination. The amount of DNA is sufficiently represented by the PI fluorescence to be able to distinguish between eu- and polyploid neurons.
机译:在阿尔茨海默病患者的神经元(Ad)患者的细胞周期重新进入以及多倍体的迹象中,表明神经元的整体或部分神经元在死亡前重复,但没有发起有丝分裂细胞DNA含量保持四倍体。结论是,这种不平衡是广告中神经元损失的直接原因。手动计数多倍体细胞可能但耗时,并且可能统计学上不足。本研究的目的是开发一种自动化方法,可检测激光扫描细胞仪(LSC)的神经元DNA含量异常。福尔曼固定的AD患者的血液固定脑组织的汞和对照受试者用抗细胞周期蛋白B和抗 - Neun抗体。使用Cy5-和Cy2-缀合的二抗和生物素链霉抗生物素蛋白或酪蛋白信号扩增进行免疫标签。在碘化钛(PI)(50μg/ ml)中孵育20μm厚度的端部,并在载玻片上覆盖。为了通过LSC PI进行分析,用作触发器。对Cyclin B表达分析了NeUN表达被NeUN表达鉴定为神经元的细胞。获得至少10,000个神经元的每个样本数据。在冷冻脑切片中,LSC可以自动定量核DNA的量。可以分析DNA倍倍增性以及细胞周期分布。可以扫描大量神经元,测量持续时间短于手动检查。 DNA的量由PI荧光充分表示,以能够区分Eu-和多倍体神经元。

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