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Computer Simulation and Additive-Based Refolding Process of Cysteine-Rich Proteins: VEGF-A as a Model
Authors:Mohsen Khaki  Ali Ganji  Hamid Abtahi  Ghasem Mosayebi  Maryam Baazm  Shabnam Sadoogh Abbasian  Ali Hatef Salmanian
Institution:1.Molecular and Medicine Research Center,Arak University of Medical Sciences,Arak,Iran;2.Department of Microbiology and Immunology, School of Medicine, Molecular and Medicine Research Center,Arak University of Medical Sciences,Arak,Iran;3.Department of Anatomy,Arak University of Medical Sciences,Arak,Iran;4.National Institute for Genetic Engineering and Biotechnology,Tehran,Iran
Abstract:Refolding of cysteine-rich protein for establishing native conformation and a biologically active form is the most challenging step in recombinant protein synthesis. In this study, expressed vascular endothelial growth factor-A (VEGF-A), as a cysteine-rich protein, in a prokaryotic expression cell was refolded based on computer simulation technique and multiple chemical additive-based buffers to recover its biologically active form. For this purpose, cloned and expressed VEGF-A in Escherichia coli BL21 (DE3) was purified and dialyzed by a basic buffer containing nine diverse chemical additives. In parallel with the evaluations of the applied additives, professional computer simulation software was also used. The activity of refolded protein was evaluated in differentiation of mesenchymal stem cells (MSCs) to the endothelial cells (ECs). The results showed that dialyzing the produced recombinant VEGF-A in chemical additive-based buffers containing cysteine, 1, 4-dithiothreitol (DTT), arginine, and Triton X-100 led to efficient VEGF-A refolding. The results of flowcytometry analysis indicated that CD31 and CD144 as the specific ECs markers in VEGF-A treated MSCs were 31 and 73%, respectively. Protein refolding method using chemical additive-based buffers containing cysteine, DTT, arginine and Triton X-100 was the best accessible technique for refolding cysteine-rich recombinant VEGF-A.
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