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Biological and Technical Variables Affecting Immunoassay Recovery of Cytokines from Human Serum and Simulated Vaginal Fluid: A Multicenter Study

机译:影响从人血清和模拟阴道液中细胞因子免疫测定回收率的生物学和技术变量:多中心研究

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The increase of proinflammatory cytokines in vaginal secretions may serve as a surrogate marker of unwanted inflammatory reaction to microbicide products topically applied for the prevention of sexually transmitted diseases, including HIV-1. Interleukin (IL)-1beta and IL-6 have been proposed as indicators of inflammation and increased risk of HIV-1 transmission; however, the lack of information regarding detection platforms optimal for vaginal fluids and interlaboratory variation limit their use for microbicide evaluation and other clinical applications. This study examines fluid matrix variants relevant to vaginal sampling techniques and proposes a model for interlaboratory comparisons across current cytokine detection technologies. IL-1beta and IL-6 standards were measured by 12 laboratories in four countries, using 14 immunoassays and four detection platforms based on absorbance, chemiluminescence, electrochemiluminescence, and fluorescence. International reference preparations of cytokines with defined biological activity were spiked into (1) a defined medium simulating the composition of human vaginal fluid at pH 4.5 and 7.2, (2) physiologic salt solutions (phosphate-buffered saline and saline) commonly used for vaginal lavage sampling in clinical studies of cytokines, and (3) human blood serum. Assays were assessed for reproducibility, linearity, accuracy, and significantly detectable fold difference in cytokine level. Factors with significant impact on cytokine recovery were determined by Kruskal-Wallis analysis of variance with Dunn's multiple comparison test and multiple regression models. All assays showed acceptable intra-assay reproducibility; however, most were associated with significant interlaboratory variation. The smallest reliably detectable cytokine differences (P < 0.05) derived from pooled interlaboratory data varied from 1.5- to 26-fold depending on assay, cytokine, and matrix type. IL-6 but not IL-1beta determinations were lower in both saline and phosphate-buffered saline as compared to vaginal fluid matrix, with no significant effect of pH. The (electro) chemiluminescence-based assays were most discriminative and consistently detected <2-fold differences within each matrix type. The Luminex-based assays were less discriminative with lower reproducibility between laboratories. These results suggest the need for uniform vaginal sampling techniques and a better understanding of immunoassay platform differences and cross-validation before the biological significance of cytokine variations can be validated in clinical trials. This investigation provides the first standardized analytic approach for assessing differences in mucosal cytokine levels and may improve strategies for monitoring immune responses at the vaginal mucosal interface.
机译:阴道分泌物中促炎细胞因子的增加可能是对局部应用杀微生物剂产品(包括HIV-1)的有害发炎反应的替代标志。已经提出白介素(IL)-1β和IL-6可作为炎症和增加HIV-1传播风险的指标。然而,缺乏有关阴道液体最佳检测平台和实验室间变异的信息,限制了其在杀菌剂评估和其他临床应用中的应用。这项研究检查了与阴道采样技术有关的流体基质变异,并提出了一种用于跨细胞因子检测的实验室间比较模型。 IL-1beta和IL-6标准品由四个国家的12个实验室使用吸光度,化学发光,电化学发光和荧光的14种免疫测定和4种检测平台进行了测量。将具有定义的生物学活性的细胞因子的国际参考制剂掺入(1)在pH 4.5和7.2下模拟人阴道液成分的确定培养基中,(2)常用用于阴道灌洗的生理盐溶液(磷酸盐缓冲液和盐水)在细胞因子的临床研究中进行采样,以及(3)人血清。评估了细胞因子水平的可重复性,线性,准确性和可检测的倍数差异。使用Dunn的多重比较检验和多重回归模型,通过Kruskal-Wallis方差分析确定对细胞因子恢复具有重大影响的因素。所有测定均显示可接受的测定内重现性;但是,大多数与实验室间的显着差异有关。根据化验间,细胞因子和基质类型的不同,从实验室间汇总数据得出的最小可靠检测的细胞因子差异(P <0.05)在1.5倍至26倍之间变化。与阴道液基质相比,盐水和磷酸盐缓冲液中的IL-6含量测定均较低,但IL-1β测定值较低,且pH值无明显影响。基于(电子)化学发光的测定法具有最高的判别力,并且在每种基质类型中均能检测到<2倍的差异。基于Luminex的测定法的判别性较低,实验室之间的再现性较低。这些结果表明,在临床试验中可以验证细胞因子变异的生物学意义之前,需要统一的阴道采样技术以及对免疫测定平台差异和交叉验证的更好理解。这项研究提供了第一个标准化的分析方法,用于评估粘膜细胞因子水平的差异,并且可能会改善监测阴道粘膜界面免疫反应的策略。

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