Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions

BACKGROUND: Overexpression of CD20 protein on the surface of B cells in lymphoma can be targeted by several anti-CD20 molecules. The development of accessible interactive epitopes is more favorable than the full-length transmembrane CD20 in the affinity assessment of anti-CD20 monoclonal antibodies...

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Autores principales: Damough, Shadi, Alizadeh, Reyhaneh, Komijani, Samira, Shirin, Mahsa, Adeli, Ahmad, Mafakher, Ladan, Mahboudi, Fereidoun, Talebkhan Garoosi, Yeganeh
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Brieflands 2023
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10024333/
https://www.ncbi.nlm.nih.gov/pubmed/36942068
http://dx.doi.org/10.5812/ijpr-134267
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author Damough, Shadi
Alizadeh, Reyhaneh
Komijani, Samira
Shirin, Mahsa
Adeli, Ahmad
Mafakher, Ladan
Mahboudi, Fereidoun
Talebkhan Garoosi, Yeganeh
author_facet Damough, Shadi
Alizadeh, Reyhaneh
Komijani, Samira
Shirin, Mahsa
Adeli, Ahmad
Mafakher, Ladan
Mahboudi, Fereidoun
Talebkhan Garoosi, Yeganeh
author_sort Damough, Shadi
collection PubMed
description BACKGROUND: Overexpression of CD20 protein on the surface of B cells in lymphoma can be targeted by several anti-CD20 molecules. The development of accessible interactive epitopes is more favorable than the full-length transmembrane CD20 in the affinity assessment of anti-CD20 monoclonal antibodies (mAbs). METHODS: The sequence of these epitopes was extracted, and the effects of different linker peptides and the location of histidine (His)-tag were computationally analyzed. The impact of thioredoxin (Trx)-tag on the folding of the selected construct and its interaction with rituximab was further investigated. The two final expression cassettes were expressed in Escherichia coli after optimization of culture conditions for incubation temperature, post-induction time, optical density at the induction time, and concentration of the inducer. ELISA evaluated the binding affinity of rituximab towards the recombinant proteins. RESULTS: By homology modeling studies, C-terminal His-tagged structures represented more desirable folded structures. Validation of the models revealed that CD20 extracellular domain linked by the G(4)S polypeptide had better stereochemical quality and structural compatibility. It was selected due to its more effective interaction with rituximab showing the highest dissociation constant of 5.8E-09M, which improved after the fusion of Trx-tag (7.1E-10M). The most influential parameters in the expression of the two selected proteins were post-induction temperature and optical density at the induction time. Homemade ELISA assays revealed a slightly higher affinity of rituximab towards the Trx-CD20 protein than the CD20/G(4)S molecule. CONCLUSIONS: Experimental in vitro studies confirmed the computationally calculated affinity of rituximab towards the two designed CD20 constructs. Also, the cell-based binding assessment of anti-CD20 mAbs could be substituted by the engineered extracellular domain of human CD20 protein.
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spelling pubmed-100243332023-03-19 Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions Damough, Shadi Alizadeh, Reyhaneh Komijani, Samira Shirin, Mahsa Adeli, Ahmad Mafakher, Ladan Mahboudi, Fereidoun Talebkhan Garoosi, Yeganeh Iran J Pharm Res Research Article BACKGROUND: Overexpression of CD20 protein on the surface of B cells in lymphoma can be targeted by several anti-CD20 molecules. The development of accessible interactive epitopes is more favorable than the full-length transmembrane CD20 in the affinity assessment of anti-CD20 monoclonal antibodies (mAbs). METHODS: The sequence of these epitopes was extracted, and the effects of different linker peptides and the location of histidine (His)-tag were computationally analyzed. The impact of thioredoxin (Trx)-tag on the folding of the selected construct and its interaction with rituximab was further investigated. The two final expression cassettes were expressed in Escherichia coli after optimization of culture conditions for incubation temperature, post-induction time, optical density at the induction time, and concentration of the inducer. ELISA evaluated the binding affinity of rituximab towards the recombinant proteins. RESULTS: By homology modeling studies, C-terminal His-tagged structures represented more desirable folded structures. Validation of the models revealed that CD20 extracellular domain linked by the G(4)S polypeptide had better stereochemical quality and structural compatibility. It was selected due to its more effective interaction with rituximab showing the highest dissociation constant of 5.8E-09M, which improved after the fusion of Trx-tag (7.1E-10M). The most influential parameters in the expression of the two selected proteins were post-induction temperature and optical density at the induction time. Homemade ELISA assays revealed a slightly higher affinity of rituximab towards the Trx-CD20 protein than the CD20/G(4)S molecule. CONCLUSIONS: Experimental in vitro studies confirmed the computationally calculated affinity of rituximab towards the two designed CD20 constructs. Also, the cell-based binding assessment of anti-CD20 mAbs could be substituted by the engineered extracellular domain of human CD20 protein. Brieflands 2023-02-15 /pmc/articles/PMC10024333/ /pubmed/36942068 http://dx.doi.org/10.5812/ijpr-134267 Text en Copyright © 2023, Author(s) https://creativecommons.org/licenses/by-nc/4.0/This is an open-access article distributed under the terms of the Creative Commons Attribution-NonCommercial 4.0 International License (http://creativecommons.org/licenses/by-nc/4.0/ (https://creativecommons.org/licenses/by-nc/4.0/) ) which permits copy and redistribute the material just in noncommercial usages, provided the original work is properly cited.
spellingShingle Research Article
Damough, Shadi
Alizadeh, Reyhaneh
Komijani, Samira
Shirin, Mahsa
Adeli, Ahmad
Mafakher, Ladan
Mahboudi, Fereidoun
Talebkhan Garoosi, Yeganeh
Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions
title Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions
title_full Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions
title_fullStr Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions
title_full_unstemmed Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions
title_short Computational and Experimental Evaluation of Linker Peptides and Thioredoxin Fusion Tag in CD20-rituximab Specific Interactions
title_sort computational and experimental evaluation of linker peptides and thioredoxin fusion tag in cd20-rituximab specific interactions
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10024333/
https://www.ncbi.nlm.nih.gov/pubmed/36942068
http://dx.doi.org/10.5812/ijpr-134267
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