ELISA validation approach for the detection of anti-saccharomyces cerevisiae antibodies in patients treated with biopharmaceutical heberprot-P®

M. P. Bernal, Carlos Hernández, Magalis Delgado, M. Izquierdo, Ileana Rosales, E. Pérez
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Abstract

This work describes the validation of an enzyme-linked immunosorbent assay (ELISA) for detection of anti-Saccharomyces cerevisiae antibodies (ASCA) in diabetic patients with foot ulcers, after the treatment with Heberprot-P®. Validation followed regulatory guidelines of US FDA and European Medicine Agency. Minimum required dilution of samples and quality controls were defined using pools of sera from diabetic patients and from healthy donors. Parameters such as cut point, specificity, precision, selectivity, robustness and sample stability were analyzed. The repeatability and intermediate precision percent ranged between 7.93-10.61% and 7.93-11.43 %, respectively, indicating low intra- and inter-assay variation. The specificity was proved by background noise suppression, reaching 100% of inhibition as strong criterion for the specificity of the immunoassay. The validated ELISA is a reliable tool for ASCA detection in human serum after the administration of Heberprot-P®, in order to find immunological reactions associated with latent contamination by host cell proteins from Saccharomyces cerevisiae.
ELISA验证方法检测接受生物药物heberprot-P®治疗的患者中的抗酿酒酵母抗体
这项工作描述了用Heberprot-P®治疗后,酶联免疫吸附试验(ELISA)检测糖尿病足溃疡患者抗酿酒酵母抗体(ASCA)的验证。验证遵循美国食品药品监督管理局和欧洲药品管理局的监管指南。使用来自糖尿病患者和健康供体的血清库来定义样品的最低所需稀释度和质量控制。分析了切点、特异性、精密度、选择性、稳健性和样品稳定性等参数。重复性和中间精密度百分比分别在7.93-10.61%和7.93-11.43%之间,表明批内和批间变异较小。背景噪声抑制证明了其特异性,抑制率达到100%,是免疫测定特异性的有力标准。经验证的ELISA是一种可靠的工具,用于在服用Heberprot-P®后检测人类血清中的ASCA,以发现与酿酒酵母宿主细胞蛋白潜在污染相关的免疫反应。
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