Standardization of flow cytometric detection of antigen expression

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS
Linhua Tian, Aaron R. Nelson, Tyler Lowe, Linda Weaver, Constance Yuan, Hao-Wei Wang, Paul DeRose, Maryalice Stetler-Stevenson, Lili Wang
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引用次数: 0

Abstract

Since response to antigen-based immunotherapy relies upon the level of tumor antigen expression we developed an antigen quantification assay using ABC values. Antigen quantification as a clinical assay requires methods for quality control and for interlaboratory and inter-cytometer platform standardization. A single lot of Cytotrol™ Lyophilized Control Cells (Beckman Coulter) used for all studies. The variability in antigen quantification across 4 different instrument platforms in 2 separate laboratories was evaluated. The effect of the antibody clone utilized, importance of custom 1:1 molar ratio (fluorophore to protein, F/P) verses off-the-shelf antibodies, and QuantiBrite PE calibration verses linearity calibration combined with a single point scale transformation with CD4 as reference were determined. Use of single lot control cells allowed validation of reproducibility between flow cytometer platforms and laboratories and allowed assessment of different antibody lots, cocktail preparation, and different antibody clones. Off the shelf antibody preparations provide reproducible estimates of antigen density, however custom 1:1 unimolar antibody preparations should be utilized for definitive measurement of antigen expression.Geometric Mean fluorescent Intensity (GeoMFI) was not comparable across instruments and inter-laboratory. The use of CD4 as the reference marker can minimize variability in ABC values. Comparable antigen quantification is vital in managing patients receiving antigen-based immunotherapy. If this assay is to be utilized in a clinical setting, quality control methods have to be instituted to assure reproducibility and allow validation across laboratories. We have demonstrated that use of a lyophilized cell control is highly valuable in achieveing these goals.

流式细胞仪检测抗原表达的标准化
由于对基于抗原的免疫疗法的反应取决于肿瘤抗原的表达水平,我们开发了一种使用 ABC 值的抗原定量检测方法。作为一种临床检测方法,抗原定量需要质量控制以及实验室间和细胞计数器间平台标准化的方法。所有研究都使用单一批次的 Cytotrol™ 冻干对照细胞(Beckman Coulter)。评估了 2 个独立实验室中 4 种不同仪器平台的抗原定量变异性。确定了所使用的抗体克隆的影响、定制 1:1 摩尔比(荧光团与蛋白质,F/P)与现成抗体的重要性、QuantiBrite PE 校准与线性校准(结合以 CD4 为参考的单点比例转换)的对比。使用单批次对照细胞可验证流式细胞仪平台和实验室之间的可重复性,并可对不同批次抗体、鸡尾酒制备和不同抗体克隆进行评估。现成的抗体制剂可提供可重复的抗原密度估计值,但要明确测量抗原表达,应使用定制的 1:1 单摩尔抗体制剂。使用 CD4 作为参考标记可最大限度地减少 ABC 值的变化。可比较的抗原定量对于管理接受抗原免疫疗法的患者至关重要。如果要在临床环境中使用这种检测方法,就必须制定质量控制方法,以确保可重复性,并允许在不同实验室之间进行验证。我们已经证明,使用冻干细胞对照对实现这些目标非常有价值。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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