多中心验证尿液 CXCL10 检测在肾移植中的非侵入性监测作用。
Multicenter Validation of a Urine CXCL10 Assay for Noninvasive Monitoring of Renal Transplants.
机构信息
Department of Internal Medicine and Immunology, University of Manitoba, Winnipeg, Canada.
Transplant Manitoba, Shared Health Manitoba, Winnipeg, Canada.
出版信息
Transplantation. 2023 Jul 1;107(7):1630-1641. doi: 10.1097/TP.0000000000004554. Epub 2023 Jun 20.
BACKGROUND
Urine CXCL10 (C-X-C motif chemokine ligand 10, interferon gamma-induced protein 10 [IP10]) outperforms standard-of-care monitoring for detecting subclinical and early clinical T-cell-mediated rejection (TCMR) and may advance TCMR therapy development through biomarker-enriched trials. The goal was to perform an international multicenter validation of a CXCL10 bead-based immunoassay (Luminex) for transplant surveillance and compare with an electrochemiluminescence-based (Meso Scale Discovery [MSD]) assay used in transplant trials.
METHODS
Four laboratories participated in the Luminex assay development and evaluation. Urine CXCL10 was measured by Luminex and MSD in 2 independent adult kidney transplant trial cohorts (Basel and TMCT04). In an independent test and validation set, a linear mixed-effects model to predict (log 10 -transformed) MSD CXCL10 from Luminex CXCL10 was developed to determine the conversion between assays. Net reclassification was determined after mathematical conversion.
RESULTS
The Luminex assay was precise, with an intra- and interassay coefficient of variation 8.1% and 9.3%; showed modest agreement between 4 laboratories (R 0.96 to 0.99, P < 0.001); and correlated with known CXCL10 in a single- (n = 100 urines, R 0.94 to 0.98, P < 0.001) and multicenter cohort (n = 468 urines, R 0.92, P < 0.001) but the 2 assays were not equivalent by Passing-Bablok regression. Linear mixed-effects modeling demonstrated an intercept of -0.490 and coefficient of 1.028, showing Luminex CXCL10 are slightly higher than MSD CXCL10, but the agreement is close to 1.0. After conversion of the biopsy thresholds, the decision to biopsy would be changed for only 6% (5/85) patients showing acceptable reclassification.
CONCLUSIONS
These data demonstrate this urine CXCL10 Luminex immunoassay is robust, reproducible, and accurate, indicating it can be readily translated into clinical HLA laboratories for serial posttransplant surveillance.
背景
尿液 CXCL10(C-X-C 基序趋化因子配体 10,干扰素 γ 诱导蛋白 10 [IP10])在检测亚临床和早期 T 细胞介导的排斥反应(TCMR)方面优于标准护理监测,并且可以通过生物标志物富集试验来推进 TCMR 治疗的发展。目的是对基于 CXCL10 珠的免疫分析(Luminex)进行国际多中心验证,用于移植监测,并与移植试验中使用的基于电化学发光的(Meso Scale Discovery [MSD])测定法进行比较。
方法
四个实验室参与了 Luminex 测定法的开发和评估。在两个独立的成人肾移植试验队列(巴塞尔和 TMCT04)中,通过 Luminex 和 MSD 测量尿液 CXCL10。在一个独立的测试和验证集中,开发了一种线性混合效应模型,以预测(对数 10 转换)MSD CXCL10 来自 Luminex CXCL10,以确定测定法之间的转换。通过数学转换后确定净再分类。
结果
Luminex 测定法精确,日内和日间变异系数分别为 8.1%和 9.3%;在四个实验室之间显示出适度的一致性(R 0.96 至 0.99,P <0.001);并且与单个(n = 100 尿液,R 0.94 至 0.98,P <0.001)和多中心队列(n = 468 尿液,R 0.92,P <0.001)中的已知 CXCL10 相关,但通过通过 - Bablok 回归,两种测定法并不等效。线性混合效应模型显示截距为-0.490,系数为 1.028,表明 Luminex CXCL10 略高于 MSD CXCL10,但一致性接近 1.0。在转换活检阈值后,只有 6%(5/85)的患者活检决定会发生变化,表明可接受的重新分类率为 6%。
结论
这些数据表明,这种尿液 CXCL10 Luminex 免疫分析具有稳健、可重复和准确的特点,表明它可以很容易地转化为临床 HLA 实验室,用于移植后的连续监测。
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