Validation of suPAR turbidimetric assay on Cobas® (c502 and c702) and comparison to suPAR ELISA

苏帕 浊度法 重复性 色谱法 罗氏诊断公司 免疫分析 检出限 医学 化学 免疫学 内科学 抗体 尿激酶受体 尿激酶
作者
Thor Aage Skovsted,Eva Rabing Brix Petersen,Maj-Britt Fruekilde,Andreas Kristian Pedersen,Tomasz Pielak,Jesper Eugen‐Olsen
出处
期刊:Scandinavian Journal of Clinical & Laboratory Investigation [Taylor & Francis]
卷期号:80 (4): 327-335 被引量:12
标识
DOI:10.1080/00365513.2020.1741674
摘要

suPAR is a plasma marker of chronic inflammation, and an elevated suPAR is consistently associated with worse outcome in a variety of clinical conditions. Quantification of suPAR is useful for determining patient risk in triage, but there is no fast automatized method for quick determination of suPAR. We developed and validated a rapid latex particle-enhanced turbidimetric immunoassay for quantification of plasma suPAR on the c502 and the c702 Roche Cobas® 8000 measurment systems. The turbidimetric assay was validated against the suPARnostic® ELISA (ViroGates, Denmark). This validation demonstrates suPAR can be analysed by turbidimetry giving very similar results (<15% difference) compared to the ELISA method and the observed correlations (n = 103) were strong, r > 0.95. Roche Cobas® 8000 instruments demonstrated repeatability and repoducibility, CV % at 3.4–4.1 and 5.7–11.4, respectively. The estimated limit of detection was 1.30 µg/L and 1.31 µg/L for the Cobas® c502 and c702, respectively. Dilution tests showed linearity of suPAR from 1.8 to 26.5 μg/L. The acceptable concentrations of Bilirubin, Intralipid and Hemoglobin, were 350 µmol/L, 3.3 g/L and 1.4 g/L, respectively. suPAR can be quantified reproducibly within 10 min using a turbidimetry assay. This assay is faster than ELISA with similar results, making it suitable for clinical routine analysis.

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