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抗胸腺基质淋巴细胞生成素纳米抗体的高性能生产工艺开发与放大

High performance production process development and scale-up of an anti-TSLP nanobody.

作者信息

Li Xiaofei, Qiao Peng, Zhang Yicai, Liu Guoxin, Zhu Min, Gai Junwei, Wan Yakun

机构信息

Shanghai Novamab Biopharmaceuticals Co., Ltd., Shanghai, China.

Shanghai Novamab Biopharmaceuticals Co., Ltd., Shanghai, China.

出版信息

Protein Expr Purif. 2024 Jun;218:106441. doi: 10.1016/j.pep.2024.106441. Epub 2024 Feb 16.

Abstract

Nanobodies (Nbs) represent a class of single-domain antibodies with great potential application value across diverse biotechnology fields, including therapy and diagnostics. Thymic Stromal Lymphopoietin (TSLP) is an epithelial cell-derived cytokine, playing a crucial role in the regulation of type 2 immune responses at barrier surfaces such as skin and the respiratory/gastrointestinal tract. In this study, a method for the expression and purification of anti-TSLP nanobody (Nb3341) was established at 7 L scale and subsequently scaled up to 100 L scale. Key parameters, including induction temperature, methanol feed and induction pH were identified as key factors by Plackett-Burman design (PBD) and were optimized in 7 L bioreactor, yielding optimal values of 24 °C, 8.5 mL/L/h and 6.5, respectively. Furthermore, Diamond Mix-A and Diamond MMC were demonstrated to be the optimal capture and polishing resins. The expression and purification process of Nb3341 at 100L scale resulted in 22.97 g/L titer, 98.7% SEC-HPLC purity, 95.7% AEX-HPLC purity, 4 ppm of HCP content and 1 pg/mg of HCD residue. The parameters of the scaling-up process were consistent with the results of the optimized process, further demonstrating the feasibility and stability of this method. This study provides a highly promising and competitive approach for transitioning from laboratory-scale to commercial production-scale of nanobodies.

摘要

纳米抗体(Nbs)是一类单域抗体,在包括治疗和诊断在内的多种生物技术领域具有巨大的潜在应用价值。胸腺基质淋巴细胞生成素(TSLP)是一种上皮细胞衍生的细胞因子,在皮肤和呼吸道/胃肠道等屏障表面的2型免疫反应调节中起关键作用。在本研究中,建立了一种7升规模表达和纯化抗TSLP纳米抗体(Nb3341)的方法,随后扩大到100升规模。通过Plackett-Burman设计(PBD)确定诱导温度、甲醇进料和诱导pH等关键参数为关键因素,并在7升生物反应器中进行优化,分别得到最佳值24℃、8.5毫升/升/小时和6.5。此外,Diamond Mix-A和Diamond MMC被证明是最佳的捕获和精制树脂。100升规模的Nb3341表达和纯化过程产生了22.97克/升的滴度、98.7%的尺寸排阻色谱-高效液相色谱(SEC-HPLC)纯度、95.7%的阴离子交换色谱-高效液相色谱(AEX-HPLC)纯度、4 ppm的宿主细胞蛋白(HCP)含量和1 pg/mg的人源化抗体片段(HCD)残留。放大过程的参数与优化过程的结果一致,进一步证明了该方法的可行性和稳定性。本研究为纳米抗体从实验室规模向商业生产规模的转变提供了一种极具前景和竞争力的方法。

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