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Optimized Standard Operating Procedures for the Analysis of Cerebrospinal Fluid Aβ42 and the Ratios of Aβ Isoforms Using Low Protein Binding Tubes

机译:使用低蛋白结合管分析脑脊液Aβ42和Aβ亚型比率的优化标准操作程序

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摘要

>Background: Reduced cerebrospinal fluid (CSF) concentration of amyloid-β1-42 (Aβ1-42) reflects the presence of amyloidopathy in brains of subjects with Alzheimer’s disease (AD).>Objective: To qualify the use of Aβ1-42/Aβ1-40 for improvement of standard operating procedures (SOP) for measurement of CSF Aβ with a focus on CSF collection, storage, and analysis.>Methods: Euroimmun ELISAs for CSF Aβ isoforms were used to set up a SOP with respect to recipient properties (low binding, polypropylene), volume of tubes, freeze/thaw cycles, addition of detergents (Triton X-100, Tween-20) in collection or storage tubes or during CSF analysis. Data were analyzed with linear repeated measures and mixed effects models.>Results: Optimization of CSF analysis included a pre-wash of recipients (e.g., tubes, 96-well plates) before sample analysis. Using the Aβ1-42/Aβ1-40 ratio, in contrast to Aβ1-42, eliminated effects of tube type, additional freeze/thaw cycles, or effect of CSF volumes for polypropylene storage tubes. ‘Low binding’ tubes reduced the loss of Aβ when aliquoting CSF or in function of additional freeze/thaw cycles. Addition of detergent in CSF collection tubes resulted in an almost complete absence of variation in function of collection procedures, but affected the concentration of Aβ isoforms in the immunoassay.>Conclusion: The ratio of Aβ1-42/Aβ1-40 is a more robust biomarker than Aβ1-42 toward (pre-) analytical interfering factors. Further, ‘low binding’ recipients and addition of detergent in collection tubes are able to remove effects of SOP-related confounding factors. Integration of the Aβ1-42/Aβ1-40 ratio and ‘low-binding tubes’ into guidance criteria may speed up worldwide standardization of CSF biomarker analysis.
机译:>背景:脑脊髓液(CSF)的淀粉样β1-42(Aβ1-42)浓度降低反映了阿尔茨海默氏病(AD)患者大脑中存在淀粉样变性。>目的:有资格使用Aβ1-42/Aβ1-40来改进用于测量脑脊液Aβ的标准操作程序(SOP),重点是脑脊液的收集,存储和分析。>方法:针对受体特性(低结合力,聚丙烯),试管体积,冷冻/融化周期,添加去污剂(Triton X-100,Tween-20),使用CSFAβ亚型的ELISA来设置SOP。管或CSF分析期间。使用线性重复测量和混合效应模型对数据进行分析。>结果:CSF分析的优化包括在样品分析之前预先清洗受体(例如试管,96孔板)。与Aβ1-42相比,使用Aβ1-42/Aβ1-40比率消除了管类型的影响,附加的冻结/解冻循环或聚丙烯存储管的CSF体积影响。等分CSF时或其他冷冻/解冻循环时,“低结合力”管可减少Aβ的损失。在脑脊液收集管中添加去污剂后,收集程序的功能几乎完全没有变化,但影响了免疫测定中Aβ亚型的浓度。>结论:Aβ1-42/Aβ1-的比率40在针对分析前干扰因子方面比Aβ1-42更强健。此外,“低结合力”受体和在收集管中添加洗涤剂能够消除与SOP相关的混杂因素的影响。将Aβ1-42/Aβ1-40比率和“低结合管”整合到指导标准中可能会加速CSF生物标志物分析的全球标准化。

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