Linhult Martin, Gülich Susanne, Gräslund Torbjörn, Simon Annelie, Karlsson Martin, Sjöberg Anna, Nord Karin, Hober Sophia
Department of Biotechnology, Royal Institute of Technology (KTH), Stockholm, Sweden.
Proteins. 2004 May 1;55(2):407-16. doi: 10.1002/prot.10616.
Staphylococcal protein A (SPA) is a cell surface protein expressed by Staphylococcus aureus. It consists of five repetitive domains. The five SPA-domains show individual interaction to the Fc-fragment as well as certain Fab-fragments of immunoglobulin G (IgG) from most mammalian species. Due to the high affinity and selectivity of SPA, it has a widespread use as an affinity ligand for capture and purification of antibodies. One of the problems with proteinaceous affinity ligands in large-scale purification is their sensitivity to alkaline conditions. SPA however, is considered relatively stable to alkaline treatment. Nevertheless, it is desirable to further improve the stability in order to enable an SPA-based affinity medium to withstand even longer exposure to the harsh conditions associated with cleaning-in-place (CIP) procedures. For this purpose, a protein engineering strategy, which was used earlier for stabilization and consists of replacing the asparagine residues, is employed. Since Z in its "nonengineered" form already has a significant tolerance to alkaline treatment, small changes in stability due to the mutations are difficult to assess. Hence, in order to enable detection of improvements regarding the alkaline resistance of the Z domain, we chose to use a bypass mutagenesis strategy using a mutated variant Z(F30A) as a surrogate framework. Z(F30A) has earlier been shown to possess an affinity to IgG that is similar to the wild-type but also demonstrates decreased structural stability. Since the contribution of the different asparagine residues to the deactivation rate of a ligand is dependent on the environment and also the structural flexibility of the particular region, it is important to consider all sensitive amino acids one by one. The parental Z-domain contains eight asparagine residues, each with a different impact on the alkaline stability of the domain. By exchanging asparagine 23 for a threonine, we were able to increase the stability of the Z(F30A) domain in alkaline conditions. Also, when grafting the N23T mutation to the Z scaffold, we were able to detect an increased tolerance to alkaline treatment compared to the native Z molecule.
葡萄球菌蛋白A(SPA)是金黄色葡萄球菌表达的一种细胞表面蛋白。它由五个重复结构域组成。这五个SPA结构域分别与大多数哺乳动物物种免疫球蛋白G(IgG)的Fc片段以及某些Fab片段相互作用。由于SPA具有高亲和力和选择性,它被广泛用作捕获和纯化抗体的亲和配体。大规模纯化中蛋白质亲和配体的一个问题是它们对碱性条件敏感。然而,SPA被认为对碱性处理相对稳定。尽管如此,为了使基于SPA的亲和介质能够承受更长时间与在位清洗(CIP)程序相关的苛刻条件,进一步提高其稳定性仍是可取的。为此,采用了一种先前用于稳定化的蛋白质工程策略,该策略包括替换天冬酰胺残基。由于“未改造”形式的Z对碱性处理已经具有显著的耐受性,因此难以评估由于突变导致的稳定性微小变化。因此,为了能够检测Z结构域在耐碱性方面的改进,我们选择使用一种旁路诱变策略,使用突变变体Z(F30A)作为替代框架。Z(F30A)先前已被证明对IgG具有与野生型相似的亲和力,但也表现出结构稳定性降低。由于不同天冬酰胺残基对配体失活速率的贡献取决于环境以及特定区域的结构灵活性,逐一考虑所有敏感氨基酸很重要。亲本Z结构域包含八个天冬酰胺残基,每个残基对结构域的碱性稳定性都有不同影响。通过将天冬酰胺23替换为苏氨酸,我们能够提高Z(F30A)结构域在碱性条件下的稳定性。此外,当将N23T突变嫁接到Z支架上时,与天然Z分子相比,我们能够检测到对碱性处理的耐受性增加。
