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大鼠抗独特型单克隆抗体WN对抗B细胞淋巴瘤单克隆抗体LL2特异性的研发与评估。

Development and evaluation of the specificity of a rat monoclonal anti-idiotype antibody, WN, to an anti-B-cell lymphoma monoclonal antibody, LL2.

作者信息

Losman M J, Leung S O, Shih L B, Shevitz J, Shukla R, Haraga L, Goldenberg D M, Hansen H J

机构信息

Immunomedics, Inc., Morris Plains, New Jersey 07950, USA.

出版信息

Cancer Res. 1995 Dec 1;55(23 Suppl):5978s-5982s.

PMID:7493380
Abstract

Anti-idiotype monoclonal antibodies (Mabs) to mLL2, an anti-B-cell lymphoma and CD22-specific murine IgG2a-kappa Mab, were generated by hybridoma technology from splenocytes of Copenhagen rats immunized with mLL2 F(ab')2. Mab WN, an IgG2a-kappa, was selected based on its specific binding to mLL2 and not other IgG isotypes or anti-B-cell Mabs. In a radioimmunoassay, WN was found to inhibit the binding of 125I-labeled mLL2 to Raji cells and to have no effect on the binding of other B-cell-reactive antibodies. Using high performance liquid chromatography analysis, WN was shown to complex specifically with both mLL2 and mLL2 Fab'. Meanwhile, we have constructed chimeric (cLL2) and humanized (hLL2) versions of LL2. Both cLL2 and hLL2 were demonstrated to retain the original antigen specificity and affinity of mLL2 [S.O. Leung et al., Proc. Am. Assoc. Cancer Res., 2872 (abstract), 34: 481, 1993]. The specific binding of WN to either radioiodinated or peroxidase-conjugated mLL2 was inhibited in a dose-response manner, and to a similar extent by mLL2, cLL2, and hLL2. Since the mLL2 complementarity-determining regions are the only sequences common to mLL2, cLL2, and hLL2, the result confirms that WN is specific to the antigen-binding complementarity-determining regions. A WN binding assay is currently being evaluated as a substitute for the tedious, and sometimes inconsistent, Raji cell-binding assay for the determination of LL2 immunoreactivity. In conclusion, we have developed an anti-idiotype Mab, WN, to mLL2. Its potential use as a surrogate antigen for B-cell lymphoma is under investigation.

摘要

通过杂交瘤技术,用mLL2 F(ab')2免疫哥本哈根大鼠的脾细胞,制备了针对抗B细胞淋巴瘤且对CD22具有特异性的鼠源IgG2a-κ单克隆抗体mLL2的抗独特型单克隆抗体(Mabs)。基于其与mLL2的特异性结合而不与其他IgG同种型或抗B细胞单克隆抗体结合,选择了IgG2a-κ单克隆抗体WN。在放射免疫分析中,发现WN可抑制125I标记的mLL2与Raji细胞的结合,而对其他B细胞反应性抗体的结合无影响。使用高效液相色谱分析表明,WN可与mLL2和mLL2 Fab'特异性结合。同时,我们构建了LL2的嵌合型(cLL2)和人源化型(hLL2)。已证明cLL2和hLL2均保留了mLL2的原始抗原特异性和亲和力[S.O. Leung等人,《美国癌症研究协会会议论文集》,2872(摘要),34:481,1993]。WN与放射性碘化或过氧化物酶偶联的mLL2的特异性结合以剂量反应方式受到抑制,并且mLL2、cLL2和hLL2对其抑制程度相似。由于mLL2的互补决定区是mLL2、cLL2和hLL2唯一共有的序列,该结果证实WN对抗原结合互补决定区具有特异性。目前正在评估WN结合试验,以替代用于确定LL2免疫反应性的繁琐且有时不一致的Raji细胞结合试验。总之,我们已开发出针对mLL2的抗独特型单克隆抗体WN。正在研究其作为B细胞淋巴瘤替代抗原的潜在用途。

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