A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format

High throughput screenings of single chain Fv (scFv) antibody phage display libraries are currently done as soluble scFvs produced in E.coli. Due to endotoxin contaminations from bacterial cells these preparations cannot be reliably used in mammalian cell based assays. The monovalent nature and lack...

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Autores principales: Xiao, Xiaodong, Chen, Yan, Mugabe, Sheila, Gao, Changshou, Tkaczyk, Christine, Mazor, Yariv, Pavlik, Peter, Wu, Herren, Dall’Acqua, William, Chowdhury, Partha Sarathi
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4607404/
https://www.ncbi.nlm.nih.gov/pubmed/26468955
http://dx.doi.org/10.1371/journal.pone.0140691
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author Xiao, Xiaodong
Chen, Yan
Mugabe, Sheila
Gao, Changshou
Tkaczyk, Christine
Mazor, Yariv
Pavlik, Peter
Wu, Herren
Dall’Acqua, William
Chowdhury, Partha Sarathi
author_facet Xiao, Xiaodong
Chen, Yan
Mugabe, Sheila
Gao, Changshou
Tkaczyk, Christine
Mazor, Yariv
Pavlik, Peter
Wu, Herren
Dall’Acqua, William
Chowdhury, Partha Sarathi
author_sort Xiao, Xiaodong
collection PubMed
description High throughput screenings of single chain Fv (scFv) antibody phage display libraries are currently done as soluble scFvs produced in E.coli. Due to endotoxin contaminations from bacterial cells these preparations cannot be reliably used in mammalian cell based assays. The monovalent nature and lack of Fc in soluble scFvs prevent functional assays that are dependent on target cross linking and/or Fc functions. A convenient approach is to convert scFvs into scFv.Fc fusion proteins and express them in mammalian cell lines for screening. This approach is low throughput and is only taken after primary screening of monovalent scFvs that are expressed in bacteria. There is no platform at present that combines the benefits of both bacterial and mammalian expression system for screening phage library output. We have, therefore, developed a novel dual expression vector, called pSplice, which can be used to express scFv.Fc fusion proteins both in E.coli and mammalian cell lines. The hallmark of the vector is an engineered intron which houses the bacterial promoter and signal peptide for expression and secretion of scFv.Fc in E.coli. When the vector is transfected into a mammalian cell line, the intron is efficiently spliced out resulting in a functional operon for expression and secretion of the scFv.Fc fusion protein into the culture medium. By applying basic knowledge of mammalian introns and splisosome, we designed this vector to enable screening of phage libraries in a product like format. Like IgG, the scFv.Fc fusion protein is bi-valent for the antigen and possesses Fc effector functions. Expression in E.coli maintains the speed of the bacterial expression platform and is used to triage clones based on binding and other assays that are not sensitive to endotoxin. Triaged clones are then expressed in a mammalian cell line without the need for any additional cloning steps. Conditioned media from the mammalian cell line containing the fusion proteins are then used for different types of cell based assays. Thus this system retains the speed of the current screening system for phage libraries and adds additional functionality to it.
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spelling pubmed-46074042015-10-29 A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format Xiao, Xiaodong Chen, Yan Mugabe, Sheila Gao, Changshou Tkaczyk, Christine Mazor, Yariv Pavlik, Peter Wu, Herren Dall’Acqua, William Chowdhury, Partha Sarathi PLoS One Research Article High throughput screenings of single chain Fv (scFv) antibody phage display libraries are currently done as soluble scFvs produced in E.coli. Due to endotoxin contaminations from bacterial cells these preparations cannot be reliably used in mammalian cell based assays. The monovalent nature and lack of Fc in soluble scFvs prevent functional assays that are dependent on target cross linking and/or Fc functions. A convenient approach is to convert scFvs into scFv.Fc fusion proteins and express them in mammalian cell lines for screening. This approach is low throughput and is only taken after primary screening of monovalent scFvs that are expressed in bacteria. There is no platform at present that combines the benefits of both bacterial and mammalian expression system for screening phage library output. We have, therefore, developed a novel dual expression vector, called pSplice, which can be used to express scFv.Fc fusion proteins both in E.coli and mammalian cell lines. The hallmark of the vector is an engineered intron which houses the bacterial promoter and signal peptide for expression and secretion of scFv.Fc in E.coli. When the vector is transfected into a mammalian cell line, the intron is efficiently spliced out resulting in a functional operon for expression and secretion of the scFv.Fc fusion protein into the culture medium. By applying basic knowledge of mammalian introns and splisosome, we designed this vector to enable screening of phage libraries in a product like format. Like IgG, the scFv.Fc fusion protein is bi-valent for the antigen and possesses Fc effector functions. Expression in E.coli maintains the speed of the bacterial expression platform and is used to triage clones based on binding and other assays that are not sensitive to endotoxin. Triaged clones are then expressed in a mammalian cell line without the need for any additional cloning steps. Conditioned media from the mammalian cell line containing the fusion proteins are then used for different types of cell based assays. Thus this system retains the speed of the current screening system for phage libraries and adds additional functionality to it. Public Library of Science 2015-10-15 /pmc/articles/PMC4607404/ /pubmed/26468955 http://dx.doi.org/10.1371/journal.pone.0140691 Text en © 2015 Xiao et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Xiao, Xiaodong
Chen, Yan
Mugabe, Sheila
Gao, Changshou
Tkaczyk, Christine
Mazor, Yariv
Pavlik, Peter
Wu, Herren
Dall’Acqua, William
Chowdhury, Partha Sarathi
A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format
title A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format
title_full A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format
title_fullStr A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format
title_full_unstemmed A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format
title_short A Novel Dual Expression Platform for High Throughput Functional Screening of Phage Libraries in Product like Format
title_sort novel dual expression platform for high throughput functional screening of phage libraries in product like format
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4607404/
https://www.ncbi.nlm.nih.gov/pubmed/26468955
http://dx.doi.org/10.1371/journal.pone.0140691
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