Labeling and stability of radiolabeled antibody fragments by a direct 99mTc-labeling method

K.Y. Pak, M.A. Nedelman, S.H. Tam, E. Wilson, P.E. Daddona
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引用次数: 22

Abstract

The in vitro labeling and stability of 99mTc-labeled antibody Fab′ fragments prepared by a direct labeling technique were evaluated. Eight antibody fragments derived from murine IgG1 (N = 5), IgG2a (N = 2) and IgG3 (N = 1) isotypes were labeled with a preformed 99mTc-d-glucarate complex. No loss of radioactivity incorporation was observed for all the 99mTc-labeled antibody fragments after 24 h incubation at 37 °C. The 99mTc-labeled antibody fragments (IgG1, N = 2; IgG2a, N = 2; IgG3, N = 1) were stable upon challenge with DTPA, EDTA or acidic pH. Furthermore, using the affinity chromatography technique, two of the 99mTc-labeled antibody fragments displayed no loss of immunoreactivity after prolonged incubation in phosphate buffer up to 24 h at 37 °C. The bonding between 99mTc and antibody fragments was elucidated by challenging with a diamide ditholate (N2S2) compound. The Fab′ with IgG2a isotype displayed tighter binding to 99mTc in comparison to the Fab′ from IgG1 and IgG3 isotype in N2S2 challenge and incubation with human plasma. The in vivo biodistribution of five 99mTc-labeled fragments were evaluated in normal mice. In conclusion, the direct labeling method allows stable 99mTc labeling of antibody fragments from three of the major murine isotypes.

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直接99mtc标记法对放射性标记抗体片段的标记和稳定性
对直接标记技术制备的99mtc标记抗体Fab’片段的体外标记性和稳定性进行了评价。来自小鼠IgG1 (N = 5)、IgG2a (N = 2)和IgG3 (N = 1)同型的8个抗体片段用预形成的99mtc -d-葡聚糖复合物标记。在37℃孵育24小时后,所有99mtc标记的抗体片段均未观察到放射性掺入损失。99mtc标记的抗体片段(IgG1, N = 2;IgG2a, N = 2;IgG3, N = 1)在DTPA, EDTA或酸性ph下均稳定。此外,使用亲和层析技术,在磷酸盐缓冲液中37°C孵育24小时后,99mtc标记的两个抗体片段未显示免疫反应性损失。99mTc与抗体片段之间的结合通过二胺二硫酸酯(N2S2)化合物的挑战被阐明。与IgG1和IgG3同型的Fab’相比,IgG2a同型的Fab’在N2S2攻毒和人血浆培养中与99mTc的结合更紧密。对5个99mtc标记片段在正常小鼠体内的生物分布进行了评价。总之,直接标记方法可以稳定地对来自三种主要小鼠同型的抗体片段进行99mTc标记。
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