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使用流式细胞术和细胞追踪测速技术对三种癌症相关抗原的抗体结合进行表征。

Characterization of antibody binding to three cancer-related antigens using flow cytometry and cell tracking velocimetry.

作者信息

Chosy E Julia, Nakamura Masayuki, Melnik Kristie, Comella Kristin, Lasky Larry C, Zborowski Maciej, Chalmers Jeffrey J

机构信息

Department of Chemical Engineering, Ohio State University, 125 Koffolt Laboratories, 140 West 19th Avenue, Columbus, Ohio 43210, USA.

出版信息

Biotechnol Bioeng. 2003 May 5;82(3):340-51. doi: 10.1002/bit.10581.

DOI:10.1002/bit.10581
PMID:12599261
Abstract

Proper antibody labeling is a fundamental step in the positive selection/isolation of rare cancer cells using immunomagnetic cell separation technology. Using either a two-step or single-step labeling protocol, we examined a combination of six different antibodies specific for three different antigens (epithelial specific antigen, epithelial membrane antigen, and HER-2/Neu) on two different breast cancer cell lines (HCC1954 and MCF-7). When a two-step labeling protocol was used (i.e., anti-surface marker-fluoroscein-isothiocyanate [FITC] [primary Ab], anti-FITC magnetic colloid [secondary Ab]) saturation of the primary antibody was determined using fluorescence intensity measurements from flow cytometry (FCM). The saturation of the secondary antibody (or saturation of a single-step labeling) was determined using magnetophoretic mobility measurements from cell tracking velocimetry (CTV). When the maximum magnetophoretic mobility was the primary objective, our results demonstrate that the quantities necessary for antibody saturation with respect to fluorescence intensity were generally higher than those recommended by the manufacturer. The results demonstrate that magnetophoretic mobility varies depending on the types of cell lines, primary antibodies, and concentration of secondary magnetic colloid-conjugated antibody. It is concluded that saturation studies are a vital preparatory step in any separation method involving antibody labeling, especially those that require the specificity of rare cell detection.

摘要

使用免疫磁珠细胞分离技术对稀有癌细胞进行阳性选择/分离时,正确的抗体标记是一个基本步骤。我们采用两步或一步标记方案,在两种不同的乳腺癌细胞系(HCC1954和MCF-7)上,检测了针对三种不同抗原(上皮特异性抗原、上皮膜抗原和HER-2/Neu)的六种不同抗体的组合。当采用两步标记方案时(即抗表面标志物-异硫氰酸荧光素[FITC][一抗],抗FITC磁性胶体[二抗]),使用流式细胞术(FCM)的荧光强度测量来确定一抗的饱和度。使用细胞跟踪测速法(CTV)的磁泳迁移率测量来确定二抗的饱和度(或一步标记的饱和度)。当最大磁泳迁移率是主要目标时,我们的结果表明,相对于荧光强度而言,抗体饱和所需的量通常高于制造商推荐的量。结果表明,磁泳迁移率因细胞系类型、一抗以及二抗磁性胶体偶联抗体的浓度而异。得出的结论是,饱和度研究是任何涉及抗体标记的分离方法中的一个重要准备步骤,尤其是那些需要检测稀有细胞特异性的方法。

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