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通过评估构象稳定性及其与聚集倾向的相关性,应用高通量相对化学稳定性测定法筛选治疗性蛋白质制剂。

Application of a high-throughput relative chemical stability assay to screen therapeutic protein formulations by assessment of conformational stability and correlation to aggregation propensity.

作者信息

Rizzo Joseph M, Shi Shuai, Li Yunsong, Semple Andrew, Esposito Jessica J, Yu Shenjiang, Richardson Daisy, Antochshuk Valentyn, Shameem Mohammed

机构信息

Sterile Product & Analytical Development, Bioprocess Development, Merck Research Laboratories, Kenilworth, New Jersey, 07033.

出版信息

J Pharm Sci. 2015 May;104(5):1632-40. doi: 10.1002/jps.24408. Epub 2015 Mar 10.

DOI:10.1002/jps.24408
PMID:25757872
Abstract

In this study, an automated high-throughput relative chemical stability (RCS) assay was developed in which various therapeutic proteins were assessed to determine stability based on the resistance to denaturation post introduction to a chaotrope titration. Detection mechanisms of both intrinsic fluorescence and near UV circular dichroism (near-UV CD) are demonstrated. Assay robustness was investigated by comparing multiple independent assays and achieving r(2) values >0.95 for curve overlays. The complete reversibility of the assay was demonstrated by intrinsic fluorescence, near-UV CD, and biologic potency. To highlight the method utility, we compared the RCS assay with differential scanning calorimetry and dynamic scanning fluorimetry methodologies. Utilizing C1/2 values obtained from the RCS assay, formulation rank-ordering of 12 different mAb formulations was performed. The prediction of long-term stability on protein aggregation is obtained by demonstrating a good correlation with an r(2) of 0.83 between RCS and empirical aggregation propensity data. RCS promises to be an extremely useful tool to aid in candidate formulation development efforts based on the complete reversibility of the method to allow for multiple assessments without protein loss and the strong correlation between the C1/2 data obtained and accelerated stability under stressed conditions.

摘要

在本研究中,开发了一种自动化高通量相对化学稳定性(RCS)测定法,通过该方法评估各种治疗性蛋白质,根据引入离液剂滴定后对变性的抗性来确定稳定性。展示了内在荧光和近紫外圆二色性(近紫外CD)的检测机制。通过比较多个独立测定法并使曲线叠加的r(2)值>0.95来研究测定法的稳健性。通过内在荧光、近紫外CD和生物学活性证明了该测定法的完全可逆性。为突出该方法的实用性,我们将RCS测定法与差示扫描量热法和动态扫描荧光法进行了比较。利用从RCS测定法获得的C1/2值,对12种不同的单克隆抗体制剂进行了配方排序。通过证明RCS与经验性聚集倾向数据之间的r(2)为0.83的良好相关性,获得了对蛋白质聚集长期稳定性的预测。基于该方法的完全可逆性,RCS有望成为一种极其有用的工具,有助于候选配方开发工作,从而能够在不损失蛋白质的情况下进行多次评估,并且所获得的C1/2数据与应激条件下的加速稳定性之间具有很强的相关性。

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Application of a high-throughput relative chemical stability assay to screen therapeutic protein formulations by assessment of conformational stability and correlation to aggregation propensity.通过评估构象稳定性及其与聚集倾向的相关性,应用高通量相对化学稳定性测定法筛选治疗性蛋白质制剂。
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