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人源化Lewis-Y特异性IgG抗体的赖氨酸剪切分析及其与Fc介导的效应器功能的关系。

Analysis of lysine clipping of a humanized Lewis-Y specific IgG antibody and its relation to Fc-mediated effector function.

作者信息

Antes Bernhard, Amon Sabine, Rizzi Andreas, Wiederkum Susi, Kainer Manuela, Szolar Oliver, Fido Markus, Kircheis Ralf, Nechansky Andreas

机构信息

Igeneon Immunotherapy of Cancer, Brunner Strasse 69/3, 1230 Vienna, Austria.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2007 Jun 1;852(1-2):250-6. doi: 10.1016/j.jchromb.2007.01.024. Epub 2007 Jan 26.

Abstract

During the analytical characterization of the humanized Lewis-Y specific monoclonal antibody IGN311 (IgG1/kappa) used for passive anti-cancer therapy in humans, isoelectric focusing (IEF) experiments revealed that IGN311 batches produced in serum-containing and serum-free medium, respectively, displayed different banding patterns. The additional bands in the IEF pattern correlated with additional peaks observed by subsequent cation exchange (CEX)-HPLC analysis. Since the IEF pattern is one of the specification criteria in the quality control of monoclonal antibodies and a non-matching pattern may be indicative for lot-to-lot inconsistency, this phenomenon was investigated in detail. First, we investigated whether a difference in antibody glycosylation was the cause for the observed charge heterogeneity. De-N-glycosylation experiments demonstrated that charge heterogeneity observed in the IEF pattern is not a consequence of glycosylation. In contrast, sample treatment by carboxypeptidase B, removing the carboxy-terminal lysine residues from the two heavy chains of the antibody, resulted in reduced charge heterogeneity eliminating the two most basic bands observed in IEF. These data were supported by reversed phase HPLC-MALDI-TOF-MS analysis of enzymatically cleaved peptides of the antibody as well as by carboxy-terminal sequencing of the heavy chains. It was demonstrated that the differences in the IEF banding pattern were due to lysine clipping occurring during the production of the antibody. The antibody batch produced under serum-free conditions was less affected by lysine clipping. Both antibody variants--clipped and unclipped--elicited the same potency in a complement dependent cytotoxicity (CDC) assay demonstrating that lysine clipping of IGN311 does not impair Fc-mediated effector functions.

摘要

在用于人类被动抗癌治疗的人源化Lewis-Y特异性单克隆抗体IGN311(IgG1/κ)的分析表征过程中,等电聚焦(IEF)实验表明,分别在含血清和无血清培养基中生产的IGN311批次呈现出不同的条带模式。IEF图谱中的额外条带与随后的阳离子交换(CEX)-HPLC分析中观察到的额外峰相关。由于IEF图谱是单克隆抗体制剂质量控制的规格标准之一,且不匹配的图谱可能表明批次间存在不一致性,因此对这一现象进行了详细研究。首先,我们研究了抗体糖基化差异是否是观察到的电荷异质性的原因。去N-糖基化实验表明,IEF图谱中观察到的电荷异质性不是糖基化的结果。相反,用羧肽酶B处理样品,去除抗体两条重链的羧基末端赖氨酸残基,导致电荷异质性降低,消除了IEF中观察到的两条最碱性的条带。这些数据得到了抗体酶解肽的反相HPLC-MALDI-TOF-MS分析以及重链羧基末端测序的支持。结果表明,IEF条带模式的差异是由于抗体生产过程中发生的赖氨酸剪切所致。在无血清条件下生产的抗体批次受赖氨酸剪切的影响较小。两种抗体变体——剪切型和未剪切型——在补体依赖性细胞毒性(CDC)试验中引发相同的效力,表明IGN311的赖氨酸剪切不会损害Fc介导的效应功能。

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