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In Silico Analysis, Molecular Docking, Molecular Dynamic, Cloning, Expression and Purification of Chimeric Protein in Colorectal Cancer Treatment Publisher Pubmed



Dana H1, 2 ; Chalbatani GM1 ; Gharagouzloo E1 ; Miri SR1 ; Memari F1 ; Rasoolzadeh R3 ; Zinatizadeh MR3 ; Zarandi PK3 ; Marmari V2
Authors
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Authors Affiliations
  1. 1. Cancer Research Center, Cancer Institute of Iran, Tehran University of Medical Science, Tehran, Iran
  2. 2. Department of Biology, Damghan Branch, Islamic Azad University, Damghan, Iran
  3. 3. Department of Biology, Science and Research Branch, Islamic Azad University, Tehran, Iran

Source: Drug Design# Development and Therapy Published:2020


Abstract

Introduction: Colorectal cancer (CRC) is a type of cancer in humans that leads to high mortality and morbidity. CD166 and CD326 are immunoglobulins that are associated with cell migration. These molecules are included in tumorigenesis of CRC and serve a great marker of CRC stem cells. In the present study, we devised a novel chimeric protein including the V1-domain of the CD166 and two epitopes of CD326 to use in diagnostic or therapeutic applications. Methods: In silico techniques were launched to characterize the properties and structure of the protein. We have predicted physicochemical properties, structures, stability, MHC class I binding properties and ligand-receptor interaction of this chimeric protein by means of computational bioinformatics tools and servers. The sequence of chimeric gene was optimized for expression in prokaryotic host using online tools and cloned into pET-28a plasmid. The recombinant pET28a was transformed into the E. coli BL21DE3. Expression of recombinant protein was examined by SDS-PAGE and Western blotting. Results: The designed chimeric protein retained high stability and the same immunogenicity as of the original proteins. Bioinformatics data indicated that the epitopes of the synthetic chimeric protein might induce B-cell-and T-cell-mediated immune responses. Furthermore, a gene was synthesized using the codon bias of a prokaryotic expression system. This synthetic gene expressed a bacterial expression system. The recombinant protein with molecular weights of 27kDa was expressed and confirmed by anti-his Western blot analysis. Conclusion: The designed recombinant protein may be useful as a CRC diagnostic tool and for developing a protective vaccine against CRC. © 2020 Dana et al.
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