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构建工程化Fab片段以在大肠杆菌中高效形成F(ab)2并提高体内稳定性。

Engineering Fab' fragments for efficient F(ab)2 formation in Escherichia coli and for improved in vivo stability.

作者信息

Rodrigues M L, Snedecor B, Chen C, Wong W L, Garg S, Blank G S, Maneval D, Carter P

机构信息

Department of Protein Engineering, Genetech Inc., South San Francisco, CA 94080.

出版信息

J Immunol. 1993 Dec 15;151(12):6954-61.

PMID:7903100
Abstract

We previously developed an efficient route to humanized F(ab')2 fragments by high level secretion of the Fab' arms from Escherichia coli followed by directed chemical coupling in vitro. Here the number and type of interchain linkages in F(ab')2 molecules has been modified to simplify their production and improve their serum stability. All F(ab')2 variants had comparable binding affinity for the p185HER2 Ag and antiproliferative activity against p185HER2-overexpressing tumor cells. This was anticipated since the modifications are distant from the Ag-binding loops. Replacement of a single disulfide bridge between Fab' arms with a more stable thioether bridge increased the serum permanence time in normal mice by threefold to 2.1 h. Removal of the disulfide bond between L and H chains in the thioether-bridged F(ab')2 did not affect the pharmacokinetics, suggesting that the L chain remains associated with the H chain. An additional Fab' variant containing three repeats of the motif, CysProPro, was constructed with the aim of promoting efficient formation of F(ab')2 in E. coli. This Fab' (CPP)3 variant was recovered predominantly (up to 70%) as F(ab')2 directly from fermentation cell pastes, thus circumventing the need for in vitro coupling. The F(ab')2 (CPP)3 variant has a similar serum pharmacokinetics to the thioether-bridged molecules. The improvements described here for deriving F(ab')2 fragments from E. coli should enhance the clinical potential of these molecules.

摘要

我们之前开发了一种高效的方法来制备人源化F(ab')2片段,即先通过大肠杆菌高水平分泌Fab'臂,然后在体外进行定向化学偶联。在此,我们对F(ab')2分子中链间连接的数量和类型进行了修饰,以简化其生产过程并提高其血清稳定性。所有F(ab')2变体对p185HER2抗原均具有相当的结合亲和力,并且对过表达p185HER2的肿瘤细胞具有抗增殖活性。鉴于这些修饰远离抗原结合环,这是可以预期的。用更稳定的硫醚桥取代Fab'臂之间的单个二硫键,可使正常小鼠体内的血清存留时间延长三倍,达到2.1小时。在硫醚桥连的F(ab')2中去除轻链和重链之间的二硫键并不影响药代动力学,这表明轻链仍与重链结合。另外构建了一个包含三个CysProPro基序重复序列的Fab'变体,目的是促进大肠杆菌中F(ab')2的高效形成。这种Fab'(CPP)3变体主要(高达70%)直接从发酵细胞糊中回收为F(ab')2,从而无需体外偶联。F(ab')2(CPP)3变体的血清药代动力学与硫醚桥连分子相似。本文所述的从大肠杆菌中获得F(ab')2片段的改进方法应能增强这些分子的临床应用潜力。

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