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HLA-DR结合临床IgG4抗体1D09C3的体外生物学活性是细胞聚集体破坏的结果,并且可以通过Fab臂交换消除。

The in vitro biological activity of the HLA-DR-binding clinical IgG4 antibody 1D09C3 is a consequence of the disruption of cell aggregates and can be abrogated by Fab arm exchange.

作者信息

Hansen Kerrin, Ruttekolk Ivo R, Glauner Heike, Becker Frank, Brock Roland, Hannus Stefan

机构信息

Intana Bioscience GmbH, Planegg, Germany.

出版信息

Mol Immunol. 2009 Oct;46(16):3269-77. doi: 10.1016/j.molimm.2009.07.031. Epub 2009 Aug 21.

DOI:10.1016/j.molimm.2009.07.031
PMID:19699529
Abstract

Antibodies of the IgG4 subclass, directed against cell surface antigens have received attention as therapeutic molecules due to their poor induction of the complement system. The MHC class II-directed IgG4 antibody 1D09C3 has been explored for the treatment of lymphomas. The mechanism-of-action is still controversial. Apoptosis induction following HLA-DR engagement has been proposed. However, the validity of these results has been questioned by the observation that antibodies may induce formation of cell aggregates and cell death is induced upon dispersion of these aggregates prior to the quantification of cell death by flow cytometry. Here we address the capacity of 1D09C3 to induce apoptosis in vitro, also taking account of the recently reported Fab arm exchange of IgG4 antibodies. 1D09C3 induces formation of tight cellular aggregates that can only be dispersed at the expense of massive cell damage and death. Using dual color fluorescence cross-correlation spectroscopy (FCCS) we demonstrate that also this antibody undergoes Fab arm exchange in the presence of IgG4. FCCS is a powerful technique to investigate the molecular mechanism of Fab arm exchange using minute amounts of reagents. Following exchange, the functionally monovalent 1D09C3 chimeras loose their ability to induce aggregate formation of HLA-DR-positive cells. Neither functionally monovalent nor bivalent 1D09C3 antibodies induce cell death or apoptosis in myeloma target cells, when microscopy instead of flow cytometry is employed as the analytical technique. Our results indicate that the activity of 1D09C3 in vitro may have been a consequence of assay design rather than an ability to induce HLA-DR-dependent cell death.

摘要

由于IgG4亚类抗体对补体系统的诱导作用较弱,针对细胞表面抗原的此类抗体作为治疗分子受到了关注。已对靶向MHC II类分子的IgG4抗体1D09C3进行了淋巴瘤治疗方面的探索。其作用机制仍存在争议。有人提出,HLA-DR结合后可诱导细胞凋亡。然而,这些结果的有效性受到了质疑,因为有观察发现,抗体可能会诱导细胞聚集体的形成,并且在通过流式细胞术对细胞死亡进行定量之前,这些聚集体分散时会诱导细胞死亡。在这里,我们研究了1D09C3在体外诱导细胞凋亡的能力,同时也考虑到了最近报道的IgG4抗体的Fab臂交换现象。1D09C3可诱导紧密细胞聚集体的形成,而这些聚集体只有在以大量细胞损伤和死亡为代价的情况下才能分散。我们使用双色荧光交叉相关光谱法(FCCS)证明,在有IgG4存在的情况下,这种抗体也会发生Fab臂交换。FCCS是一种利用微量试剂研究Fab臂交换分子机制的强大技术。交换后,功能单价的1D09C3嵌合体失去了诱导HLA-DR阳性细胞形成聚集体的能力。当使用显微镜而非流式细胞术作为分析技术时,功能单价和双价的1D09C3抗体均不会诱导骨髓瘤靶细胞死亡或凋亡。我们的结果表明,1D09C3在体外的活性可能是检测设计的结果,而非诱导HLA-DR依赖性细胞死亡的能力所致。

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