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一种用于在治疗性抗体的制剂开发过程中检测和表征可逆自组装的系统多技术方法。

A systematic multitechnique approach for detection and characterization of reversible self-association during formulation development of therapeutic antibodies.

机构信息

Department of Formulation Sciences, MedImmune, Gaithersburg, Maryland 20878, USA.

出版信息

J Pharm Sci. 2013 Jan;102(1):62-72. doi: 10.1002/jps.23369. Epub 2012 Nov 13.

Abstract

In addition to controlling typical instabilities such as physical and chemical degradations, understanding monoclonal antibodies' (mAbs) solution behavior is a key step in designing and developing process and formulation controls during their development. Reversible self-association (RSA), a unique solution property in which native, reversible oligomeric species are formed as a result of the noncovalent intermolecular interactions has been recognized as a developability risk with the potential to negatively impact manufacturing, storage stability, and delivery of mAbs. Therefore, its identification, characterization, and mitigation are key requirements during formulation development. Considering the large number of available analytical methods, choice of the employed technique is an important contributing factor for successful investigation of RSA. Herein, a multitechnique (dynamic light scattering, multiangle static light scattering, and analytical ultracentrifugation) approach is employed to comprehensively characterize the self-association of a model immunoglobulin G1 molecule. Studies herein discuss an effective approach for detection and characterization of RSA during biopharmaceutical development based on the capabilities of each technique, their complementarity, and more importantly their suitability for the stage of development in which RSA is investigated.

摘要

除了控制物理和化学降解等典型的不稳定性外,了解单克隆抗体(mAbs)的溶液行为是在其开发过程中设计和开发工艺和配方控制的关键步骤。可逆自组装(RSA)是一种独特的溶液性质,其中由于非共价分子间相互作用而形成天然的、可逆的寡聚体。它被认为是一种具有开发风险的物质,可能会对 mAbs 的制造、储存稳定性和输送产生负面影响。因此,在配方开发过程中,识别、表征和减轻 RSA 是关键要求。考虑到有大量可用的分析方法,所采用技术的选择是成功研究 RSA 的一个重要因素。本文采用多技术(动态光散射、多角度静态光散射和分析超速离心)方法全面表征模型免疫球蛋白 G1 分子的自组装。本文讨论了一种基于每种技术的能力、互补性以及更重要的是其适用于研究 RSA 的开发阶段的有效方法,用于在生物制药开发过程中检测和表征 RSA。

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