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开发基于稳健报告基因的 IL-5 靶向治疗性抗体生物活性测定方法。

Development of a robust reporter gene based assay for the bioactivity determination of IL-5-targeted therapeutic antibodies.

机构信息

Department of Biochemistry and Molecular Biology, The State Key Laboratory of Cancer Biology, The Fourth Military Medical University, No. 169, Changle West Road, Xi'an, Shaanxi, 710032, China; Key Laboratory of the Ministry of Health for Research on Quality and Standardization of Biotech Products, National Institutes for Food and Drug Control, No. 2, Tiantan Xili, Dongcheng District, Beijing, 100050, China.

Key Laboratory of the Ministry of Health for Research on Quality and Standardization of Biotech Products, National Institutes for Food and Drug Control, No. 2, Tiantan Xili, Dongcheng District, Beijing, 100050, China.

出版信息

J Pharm Biomed Anal. 2018 Jan 30;148:280-287. doi: 10.1016/j.jpba.2017.09.032. Epub 2017 Sep 28.

Abstract

Eosinophilic asthma is characterized by the eosinophilic inflammation with the allergen independent activation of Th2 lymphocytes. Since IL-5 plays an important role in the maturation, survival and migration of eosinophils, hence the pathogenesis of eosinophilic asthma, biotherapeutics targeting IL-5/IL-5Rα have been developed and/or marketed, including Mepolizumab, Reslizumab, and Benralizumab. Accurate determination of bioactivity is crucial for the safety and efficacy of therapeutic antibodies. The current mode of action (MOA) based method used in the quality control and stability tests for anti-IL-5 mAbs is anti-proliferation assay, which is tedious with long duration and high variation. We describe here the development and validation of a reporter gene assay (RGA), based on an IL-5-dependent TF-1 cell line variant we established that stably expresses the luciferase reporter under the control of STAT5 response elements. After careful optimization, we demonstrate the excellent specificity, precision, accuracy and linearity of the established RGA. Our study also proves that the assay is superior on precision, sensitivity and assay simplicity to the anti-proliferation assay. The established RGA is also applicable to another anti-IL-5Rα mAb. These results show for the first time that this novel RGA, based on the IL-5-IL-5R-STAT5 pathway, can be a valuable supplement to the anti-proliferation assay and employed in the bioactivity determination of anti-IL-5/anti-IL-5Rα biotherapeutics.

摘要

嗜酸性粒细胞性哮喘的特征是嗜酸性粒细胞炎症,与过敏原无关的 Th2 淋巴细胞激活。由于白细胞介素-5(IL-5)在嗜酸性粒细胞的成熟、存活和迁移中发挥重要作用,因此针对 IL-5/IL-5Rα 的生物疗法已被开发和/或上市,包括美泊利珠单抗、瑞利珠单抗和贝那利珠单抗。准确测定生物活性对于治疗性抗体的安全性和疗效至关重要。目前,用于抗 IL-5 mAb 质量控制和稳定性测试的基于作用机制(MOA)的方法是抗增殖测定法,该方法繁琐、耗时且变异性大。我们在此描述了一种报告基因测定法(RGA)的开发和验证,该方法基于我们建立的一种依赖于白细胞介素-5 的 TF-1 细胞系变体,该变体在 STAT5 反应元件的控制下稳定表达荧光素酶报告基因。经过仔细优化,我们证明了建立的 RGA 具有出色的特异性、精密度、准确性和线性度。我们的研究还证明,该测定法在精密度、灵敏度和测定简单性方面优于抗增殖测定法。该建立的 RGA 也适用于另一种抗 IL-5Rα mAb。这些结果首次表明,这种基于白细胞介素-5-白细胞介素-5 受体-STAT5 途径的新型 RGA 可以作为抗增殖测定法的有益补充,并用于抗 IL-5/抗 IL-5Rα 生物疗法的生物活性测定。

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