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Validation of an Optimized ELISA for Quantitative Assessment of Epstein-Barr Virus Antibodies from Dried Blood Spots

机译:验证优化的ELISA定量评估的eb病毒抗体干血滴

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摘要

Our objective was to validate a commercially available ELISA to measure antibody titers against Epstein-Barr virus (EBV) in dried blood spots (DBS) to replace a previously validated assay for DBS that is no longer available. We evaluated the precision, reliability, and stability of the assay for the measurement of EBV antibodies in matched plasma, fingerprick DBS, and venous blood DBS samples from 208 individuals. Effects of hematocrit and DBS sample matrix on EBV antibody determination were also investigated, and the cutoff for seropositivity in DBS was determined. A conversion equation was derived to enable comparison of results generated using this method with the former DBS method. There was a high correlation between plasma and DBS EBV antibody titers (R-2=0.93) with very little bias (-0.07 based on Bland-Altman analysis). The assay showed good linearity and did not appear to be affected by the DBS matrix, and physiological hematocrit levels had no effect on assay performance. There was reasonable agreement between DBS EBV titer estimates obtained using this assay and the previously validated assay (R-2=0.72). The commercially available ELISA assay for EBV antibody titers that we validated for use with DBS will facilitate continued investigation of EBV antibody titers in DBS.
机译:我们的目标是验证一个商业可用ELISA测定抗体滴度eb病毒(EBV)干血点(DBS)来取代先前验证测定DBS不再可用。评估的精度、可靠性和EBV的稳定性试验的测量fingerprick DBS抗体与等离子体,从208年和静脉血DBS样本个人。矩阵在巴尔病毒抗体测定也调查和血清阳性的截止在星展银行确定。推导,使生成的结果比较使用这种方法与前DBS的方法。等离子体之间有高度的相关性DBS EBV抗体滴度与非常(r2 = 0.93)基于Bland-Altman小偏差(-0.07分析)。似乎并未受到DBS矩阵,和生理比容水平没有影响在分析性能。协议DBS EBV效价估计使用这个化验和先前获得的验证试验(r2 = 0.72)。可用ELISA检测EBV抗体滴度我们使用星展银行将进行验证促进EBV的继续调查在DBS抗体滴度。

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