循环无细胞DNA在血浆和纯化形式中经过长时间的储存后产量显著下降

N. Yuwono, Mollie Ailie Acheson Boyd, C. Henry, Bonnita Werner, C. Ford, K. Warton
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引用次数: 3

摘要

目的循环DNA (cirDNA)通常是从生物银行保存不同时间的血浆中纯化出来的。在长期实验或临床试验中,血浆可以冷冻保存长达数年。因此,确定cirDNA的稳定性以确保分析时样品质量的可信度是至关重要的。我们的主要目的是确定长达2年的存储对cirDNA产量和碎片化的影响。方法我们储存了10名健康女性供体的冷冻EDTA血浆并纯化了cirDNA,然后通过qPCR和Qubit在基线和2年内定期定量cirDNA的产量。我们还比较了储存16个月后非溶血和溶血血液样本中的cirDNA水平,并测试了不同DNA提取方案参数的影响。结果保存2年以上,血浆cirDNA产量下降25.5%,纯化DNA产量下降23%,短片段比长片段损失更快。此外,cirDNA产率受血浆输入和cirDNA洗脱量的影响,但不受溶血的影响。基于cirDNA的长期研究和临床试验的设计应考虑到cirDNA在储存过程中的恶化。
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Circulating cell-free DNA undergoes significant decline in yield after prolonged storage time in both plasma and purified form
Abstract Objectives Circulating DNA (cirDNA) is generally purified from plasma that has been biobanked for variable lengths of time. In long-term experiments or clinical trials, the plasma can be stored frozen for up to several years. Therefore, it is crucial to determine the stability of cirDNA to ensure confidence in sample quality upon analysis. Our main objective was to determine the effect of storage for up to 2 years on cirDNA yield and fragmentation. Methods We stored frozen EDTA plasma and purified cirDNA from 10 healthy female donors, then quantified cirDNA yield at baseline, and at regular intervals for up to 2 years, by qPCR and Qubit. We also compared cirDNA levels in non-haemolysed and haemolysed blood samples after 16 months of storage and tested the effect of varying DNA extraction protocol parameters. Results Storage up to two years caused an annual cirDNA yield decline of 25.5% when stored as plasma and 23% when stored as purified DNA, with short fragments lost more rapidly than long fragments. Additionally, cirDNA yield was impacted by plasma input and cirDNA elution volumes, but not by haemolysis. Conclusions The design of long-term cirDNA-based studies and clinical trials should factor in the deterioration of cirDNA during storage.
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