A trimeric structural fusion of an antagonistic tumor necrosis factor-α mutant enhances molecular stability and enables facile modification

Masaki Inoue,Daisuke Ando,Haruhiko Kamada,Shintaro Taki,Mayumi Niiyama,Yohei Mukai,Takashi Tadokoro,Katsumi Maenaka,Taisuke Nakayama,Yuji Kado,Tsuyoshi Inoue,Yasuo Tsutsumi,Shin-Ichi Tsunoda

doi:10.1074/jbc.m117.779686

Abstract

Tumor necrosis factor-α (TNF) exerts its biological effect through two types of receptors, p55 TNF receptor (TNFR1) and p75 TNF receptor (TNFR2). An inflammatory response is known to be induced mainly by TNFR1, whereas an anti-inflammatory reaction is thought to be mediated by TNFR2 in some autoimmune diseases. We have been investigating the use of an antagonistic TNF mutant (TNFR1-selective antagonistic TNF mutant (R1antTNF)) to reveal the pharmacological effect of TNFR1-selective inhibition as a new therapeutic modality. Here, we aimed to further improve and optimize the activity and behavior of this mutant protein both in vitro and in vivo Specifically, we examined a trimeric structural fusion of R1antTNF, formed via the introduction of short peptide linkers, as a strategy to enhance bioactivity and molecular stability. By comparative analysis with R1antTNF, the trimeric fusion, referred to as single-chain R1antTNF (scR1antTNF), was found to retain in vitro molecular properties of receptor selectivity and antagonistic activity but displayed a marked increase in thermal stability. The residence time of scR1antTNF in vivo was also significantly prolonged. Furthermore, molecular modification using polyethylene glycol (PEG) was easily controlled by limiting the number of reactive sites. Taken together, our findings show that scR1antTNF displays enhanced molecular stability while maintaining biological activity compared with R1antTNF.

Highlights

These findings revealed that the receptor affinity and biological activity of R1antTNF were retained by scR1antTNFs despite the presence and the length of the peptide linkers within this trimeric structure
We investigated the thermal stability of scR1antTNF in vitro by using a thermal shift assay (TSA) and differential scanning calorimetry (DSC)
We previously reported that N terminus-specific monoPEGylation of R1antTNF improved in vivo stability [20, 21]

Summary

Introduction

TNF inhibitors in various molecular formats such as a neutralizing antibody (infliximab or adalimumab), soluble receptor (etanercept), or a PEGylated antibody Fab fragment (certolizumab pegol), have been clinically used as anti-TNF drugs to treat autoimmune diseases such as rheumatoid arthritis, multiple sclerosis, and ulcerative colitis [1,2,3]. These drugs elicit a highly beneficial therapeutic effect, but this treatment may lead to serious complications including bacterial or viral infection [4, 5], demyelination [6], and lupus-like syndrome [7]. There may be heterogeneous modification reactions associated with the PEGylation procedure

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