Poskute Ryte, Sankaran Praveen Kallamvalliillam, Sewell Laura, Lepore Giordana, Shrubsall Rebecca, Dewis Lydia, Watanabe Yasunori, Wong Vanessa, Pascual Fernandez Laura, Mishra Rahul, Holt Alexander, Sou Susie, Harris Claire, Moreno Rodriguez Cristina, Cankorur-Cetinkaya Ayca, Smith Jennifer, Lonska Nikola, Powell Adam, Cui Tingting, Cheeks Matthew, Lindo Viv
Analytical Sciences, BioPharmaceuticals Development, R&D, AstraZeneca, Cambridge, UK.
Analytical Sciences, BioPharmaceuticals Development, R&D, AstraZeneca, Cambridge, UK.
J Chromatogr B Analyt Technol Biomed Life Sci. 2024 Apr 15;1237:124085. doi: 10.1016/j.jchromb.2024.124085. Epub 2024 Mar 16.
Developing a knob-into-hole asymmetric bispecific IgG1 monoclonal antibody (mAb) poses manufacturing challenges due to the expression of chain pairing variants, also called mispaired species, in the desired product. The incorrect pairing of light and heavy chains could result in heterogeneous mispaired species of homodimers, heterodimers, light chain swapping, and low molecular weight species (LMWS). Standard chromatography, capillary electrophoretic, or spectroscopic methods poorly resolve these from the main variants. Here, we report a highly sensitive reverse-phase polyphenyl ultra-high-performance liquid chromatography (RP-UHPLC) method to accurately measure mispaired species of Duet mAb format, an asymmetric IgG1 bispecific mAb, for both process development and quality control analytical tests. Coupled with electrospray ionization mass spectrometry (ESI-MS), it enabled direct online characterization of mispaired species. This single direct assay detected diverse mispaired IgG-like species and LMWS. The method resolved eight disulfide bonds dissociated LMWS and three mispaired LMWS. It also resolved three different types of IgG-like mispaired species, including two homodimers and one heterodimer. The characterization and quantification simultaneously enabled the cell line selection that produces a lesser heterogeneity and lower levels of mispaired species with the desired correctly paired product. The biological activity assessment of samples with increased levels of these species quantified by the method exhibited a linear decline in potency with increasing levels of mispaired species in the desired product. We also demonstrated the utility of the technique for testing in-process intermediate materials to determine and assess downstream purification process capability in removing diverse mispaired IgG-like species and LMWS to a certain level during the downstream purification process. Our investigation demonstrates that adopting this method was vital in developing asymmetric bispecific mAb from the initial stage of cell line development to manufacturing process development. Therefore, this tool could be used in the control strategy to monitor and control mispaired species during manufacturing, thus improving the quality control of the final product.
开发一种旋钮插入孔不对称双特异性IgG1单克隆抗体(mAb)会带来制造方面的挑战,因为在目标产品中会表达链配对变体,也称为错配物种。轻链和重链的不正确配对可能导致同型二聚体、异型二聚体、轻链交换和低分子量物种(LMWS)等异质错配物种。标准色谱法、毛细管电泳法或光谱法很难将这些与主要变体区分开来。在此,我们报告了一种高灵敏度的反相聚苯基超高效液相色谱(RP-UHPLC)方法,用于准确测量Duet mAb形式(一种不对称IgG1双特异性mAb)的错配物种,用于工艺开发和质量控制分析测试。与电喷雾电离质谱(ESI-MS)联用,它能够对错配物种进行直接在线表征。这种单一直接测定法检测到了多种错配的IgG样物种和LMWS。该方法解析了八个二硫键解离的LMWS和三个错配的LMWS。它还解析了三种不同类型的IgG样错配物种,包括两个同型二聚体和一个异型二聚体。表征和定量同时实现了细胞系选择,该细胞系产生的异质性较小,错配物种水平较低,且具有所需的正确配对产品。通过该方法定量的这些物种水平增加的样品的生物活性评估显示,随着目标产品中错配物种水平的增加,效力呈线性下降。我们还证明了该技术在测试过程中间材料方面的实用性,以确定和评估下游纯化过程在下游纯化过程中将多种错配的IgG样物种和LMWS去除到一定水平的能力。我们的研究表明,采用这种方法对于从细胞系开发的初始阶段到制造工艺开发的不对称双特异性mAb的开发至关重要。因此,该工具可用于控制策略,以在制造过程中监测和控制错配物种,从而提高最终产品的质量控制。
