• Title of article

    Design and Construction of a Novel Humanized Single-Chain Variable- Fragment Antibody Against the Tumor Necrosis Factor Alpha

  • Author/Authors

    Farajzadeh, Davoud Department of Cellular and Molecular Biology - Faculty of Basic Sciences - Azarbaijan Shahid Madani University, Tabriz , Karimi-Gharigh, Sadigheh Department of Cellular and Molecular Biology - Faculty of Basic Sciences - Azarbaijan Shahid Madani University, Tabriz , Jalali-Kondori, Parisa Department of Cellular and Molecular Biology - Faculty of Basic Sciences - Azarbaijan Shahid Madani University, Tabriz , Dastmalchi, Siavoush Biotechnology Research Center and Department of Medicinal Chemistry - School of Pharmacy - Tabriz University of Medical Sciences, Tabriz

  • Pages
    12
  • From page
    308
  • To page
    319
  • Abstract
    The pro-inflammatory cytokine, TNF-α, which plays a major role in the development and persistence of inflammatory diseases, is the basis for the use of anti-TNF-α therapies. The neutralization of TNF-α or blockage of its binding to the corresponding receptor has mainly served as a therapeutic strategy against some diseases. This study aimed to investigate the production of a humanized single chain antibody (scFv) against TNF-α. Therefore, a murine monoclonal antibody, D2 mAb, was selected for humanizing by the complementarity determining region (CDR)-grafting method. Briefly, the replacement of the CDRs from D2 mAb with the specific human single chain scaffold led to the production of a novel humanized scFv mAb against human TNF-α (hD2). Cloning of hD2 into a suitable expression vector, pGEX-6P-1, resulted in the expression of a 52-kDa GST-fusion protein in E. coli, mostly in the form of inclusion bodies. The solubilization and refolding of GST-hD2 inclusion bodies was achieved with the addition of 4 M urea and subsequent dialysis to recover the fusion protein in soluble form. Then the soluble GST-hD2 was purified by affinity chromatography through immobilized glutathione. The GST pull-down experiment showed a positive interaction between GST-hD2 and TNF-α protein. Moreover, the results of an MTT assay showed that the purified GST-hD2 has TNF-α neutralizing activity (Kd of 1.03 nM) and hence hD2 has the potential to be developed into a therapeutic agent. However, more investigation is needed to elucidate the potential of in vivo TNF-α neutralizing activity of hD2 in comparison to other anti-TNF-α antibodies.
  • Keywords
    TNF-α , Single chain antibody , Affinity chromatography , Pull down , MTT assay
  • Journal title
    Astroparticle Physics
  • Serial Year
    2019
  • Record number

    2484656