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证据、操纵和终止 pH“纳米缓冲”用于单克隆抗体的定量均相清除。

Evidence, Manipulation, and Termination of pH 'Nanobuffering' for Quantitative Homogenous Scavenging of Monoclonal Antibodies.

机构信息

EMT Research Center , Institut National de la Recherche Scientifique (INRS) , Varennes , Quebec J3X 1S2 , Canada.

Faculty of Science , University of Ontario Institute of Technology , Oshawa , Ontario L1H 7K4 , Canada.

出版信息

ACS Nano. 2019 Feb 26;13(2):1019-1028. doi: 10.1021/acsnano.8b07202. Epub 2019 Jan 3.

DOI:10.1021/acsnano.8b07202
PMID:30588795
Abstract

This study demonstrates that pH-responsive polymers have a very high buffering capacity in their immediate vicinity, a phenomenon termed "nanobuffering". This can be exploited to dissociate local nanoscale pH from bulk solution pH. Herein, a series of pH-responsive polymers were conjugated to Protein-A to rationally manipulate the latter's binding affinity toward antibodies via nanobuffering ( i. e., this interaction is pH dependent), independently of bulk solution pH. Moreover, the nanobuffering effect could be terminated using low concentrations of strong ion-pairing salts, to achieve quantitative release of the antibodies from the bioconjugate. These complementary discoveries are showcased in the context of the development of a homogeneous affinity precipitation agent ( i. e., a scavenger) for the purification of polyclonal immunoglobulin G and two monoclonal antibodies from cell culture supernatant. Indeed, while bulk solution pH was used to induce precipitation of the scavenger, maintaining local nanoscale pH via nanobuffering maximized binding interaction with the antibodies. A 2:1 binding stoichiometry was observed, which was similar to that observed for native protein. The scavenger could be recycled multiple times, and the purification protocol circumvented lengthy/tedious physical purification processes typically associated with mAb manufacturing. Overall, this study provides perspectives on the local nanoscale pH near pH-responsive polymers and establishes lines of thought for predictably manipulating or even terminating nanobuffering, to control the activity of proteins.

摘要

本研究表明,pH 响应聚合物在其附近具有非常高的缓冲能力,这种现象称为“纳米缓冲”。可以利用这种特性将局部纳米级 pH 与体相溶液 pH 分离。在此,一系列 pH 响应聚合物被连接到 Protein-A 上,通过纳米缓冲(即,这种相互作用是 pH 依赖性的)来合理地操纵后者与抗体的结合亲和力,而与体相溶液 pH 无关。此外,通过使用低浓度的强离子对盐可以终止纳米缓冲效应,从而实现抗体从生物缀合物的定量释放。这些互补的发现展示在开发用于从细胞培养上清液中纯化多克隆免疫球蛋白 G 和两种单克隆抗体的均相亲和沉淀剂(即清除剂)的背景下。事实上,虽然使用体相溶液 pH 来诱导沉淀剂沉淀,但通过纳米缓冲来维持局部纳米级 pH 可最大程度地增强与抗体的结合相互作用。观察到 2:1 的结合化学计量比,与天然蛋白质观察到的相似。该清除剂可以多次回收,并且该纯化方案避免了与 mAb 制造相关的冗长/繁琐的物理纯化过程。总的来说,本研究提供了关于 pH 响应聚合物附近局部纳米级 pH 的观点,并为可预测地操纵甚至终止纳米缓冲以控制蛋白质的活性提供了思路。

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