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改进 α-突触核蛋白种子扩增测定法的方案:分析预分析和分析变量,并确定种子定量的候选参数。

Improving protocols for α-synuclein seed amplification assays: analysis of preanalytical and analytical variables and identification of candidate parameters for seed quantification.

机构信息

419170 IRCCS Istituto delle Scienze Neurologiche di Bologna , Bologna, Italy.

Department of Biomedical and Neuromotor Sciences, 9296 University of Bologna , Bologna, Italy.

出版信息

Clin Chem Lab Med. 2024 Mar 11;62(10):2001-2010. doi: 10.1515/cclm-2023-1472. Print 2024 Sep 25.

Abstract

OBJECTIVES

The effect of preanalytical and analytical factors on the α-synuclein (α-syn) seed amplification assay's (SAA) performance has not been fully explored. Similarly, there is limited knowledge about the most suitable assay protocol and kinetic parameters for misfolded α-syn seed quantification.

METHODS

We studied the effect of centrifugation, repeated freeze-thaw cycles (up to seven), delayed freezing, detergent addition, and blood contamination on the performance of the cerebrospinal fluid (CSF) α-syn SAA real-time quaking-induced conversion (RT-QuIC). Moreover, we analysed the inter- and intra-plate variability, the recombinant protein batch effect, and the RT-QuIC parameters' variability when multiple samples were run in controlled conditions. Finally, we evaluated the assay potential of quantifying α-syn seed by assessing kinetic curves in serial CSF dilutions.

RESULTS

Among tested preanalytical variables, a ≥0.01 % blood contamination and adding detergents significantly affected the RT-QuIC kinetic parameters and the number of positive replicates. Increasing the number of replicates improved result reproducibility. The number of positive replicates in serially diluted CSF samples improved discrimination between samples with high and low seeding activity, and the time to threshold (LAG) was the most reliable kinetic parameter in multiple experiment settings.

CONCLUSIONS

Preanalytical variables affecting α-syn RT-QuIC performance are limited to blood contamination and detergent addition. The number of positive replicates and the LAG are the most reliable variables for quantifying α-syn seeding activity. Their consistent measurement in serial dilution experiments, especially when associated with an increased number of sample replicates, will help to develop the α-syn RT-QuIC assay further into a quantitative test.

摘要

目的

分析前和分析因素对α-突触核蛋白(α-syn)种子扩增检测(SAA)性能的影响尚未得到充分研究。同样,对于错误折叠的α-syn 种子定量最适合的检测方案和动力学参数也知之甚少。

方法

我们研究了离心、重复冻融循环(多达 7 次)、延迟冷冻、添加去污剂以及血液污染对脑脊液(CSF)α-syn SAA 实时震颤诱导转换(RT-QuIC)的影响。此外,我们分析了板间和板内变异性、重组蛋白批间效应以及在受控条件下运行多个样本时 RT-QuIC 参数的变异性。最后,通过评估 CSF 系列稀释液中动力学曲线来评估定量 α-syn 种子的检测能力。

结果

在测试的分析前变量中,血液污染≥0.01%和添加去污剂显著影响 RT-QuIC 动力学参数和阳性重复次数。增加重复次数可提高结果的可重复性。CSF 连续稀释样本中阳性重复次数提高了高和低播种活性样本的区分能力,而时间到阈值(LAG)是多种实验设置中最可靠的动力学参数。

结论

影响 α-syn RT-QuIC 性能的分析前变量仅限于血液污染和去污剂添加。阳性重复次数和 LAG 是定量 α-syn 播种活性最可靠的变量。在连续稀释实验中对其进行一致测量,特别是与增加样本重复次数相关时,将有助于进一步将 α-syn RT-QuIC 检测发展为定量检测。

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