Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli

Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli

Recombinant antibodies and antibody fragments have become powerful tools for therapy, in vivo and in vitro diagnostics, and laboratory research. However, the production of antibody fragments in high yield for preclinical and clinical trials can be a serious bottleneck in drug discovery. This dissert...

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Main Author: Seo, Min Jeong, 1979-
Format: Others
Language:English
Published: 2012
Subjects:
Recombinant antibodies
Escherichia coli > Genetics
High throughput screening (Drug development)
Online Access:http://hdl.handle.net/2152/17756
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spelling ndltd-UTEXAS-oai-repositories.lib.utexas.edu-2152-177562015-09-20T17:09:22ZDevelopment of high throughput screening systems for the efficient production of antibody fragments in Escherichia coliSeo, Min Jeong, 1979-Recombinant antibodiesEscherichia coli--GeneticsHigh throughput screening (Drug development)Recombinant antibodies and antibody fragments have become powerful tools for therapy, in vivo and in vitro diagnostics, and laboratory research. However, the production of antibody fragments in high yield for preclinical and clinical trials can be a serious bottleneck in drug discovery. This dissertation describes the development of novel screening systems for isolating antibody fragments and alternatively, E. coli genes, that facilitate expression in E. coli. In the first part of this work, we have developed a screening system for isolating Fab mutants exhibiting 4~5 fold higher expression level at 37oC compared to the parental Fab, by utilizing the APEx 2-hybrid system and multi-color FACS as a screening tool. In the APEx 2-hybrid system, the bacterial periplasm constitutes the milieu for the association of membrane-anchored bait protein and solubly expressed, epitope-tagged prey protein. Upon disruption of the outer membrane, only prey proteins that bind to the bait remain cell-associated and are detected by flow cytometry using fluorescently labeled anti-epitope antibodies. In the second part of this work we developed a new strategy to engineer scFv that can be expressed in soluble and active form in the absence of disulfide bonds. This was achieved using a strain incapable of forming disulfide bonds in proteins expressed in its periplasm in combination with the APEx 2-hybrid system. The selected clones exhibited higher solubility, activity, and stability than that of the wild type scFv in the reducing condition of the cytoplasm. Finally, we sought to isolate E. coli gene fragments that can enhance IgG production in the periplasm of E. coli by a newly developed screening system based on soluble expression of IgG and E. coli genomic fragments. The isolated gene fragments, which are located between moeA and iaaA in the E. coli chromosome, improved the total expression of polypeptides of IgG and also assembly of IgG.text2012-09-04T16:20:36Z2012-09-04T16:20:36Z2008-082012-09-04electronichttp://hdl.handle.net/2152/17756engCopyright is held by the author. Presentation of this material on the Libraries' web site by University Libraries, The University of Texas at Austin was made possible under a limited license grant from the author who has retained all copyrights in the works.
collection NDLTD
language English
format Others
sources NDLTD
topic Recombinant antibodies
Escherichia coli--Genetics
High throughput screening (Drug development)
spellingShingle Recombinant antibodies
Escherichia coli--Genetics
High throughput screening (Drug development)
Seo, Min Jeong, 1979-
Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli
description Recombinant antibodies and antibody fragments have become powerful tools for therapy, in vivo and in vitro diagnostics, and laboratory research. However, the production of antibody fragments in high yield for preclinical and clinical trials can be a serious bottleneck in drug discovery. This dissertation describes the development of novel screening systems for isolating antibody fragments and alternatively, E. coli genes, that facilitate expression in E. coli. In the first part of this work, we have developed a screening system for isolating Fab mutants exhibiting 4~5 fold higher expression level at 37oC compared to the parental Fab, by utilizing the APEx 2-hybrid system and multi-color FACS as a screening tool. In the APEx 2-hybrid system, the bacterial periplasm constitutes the milieu for the association of membrane-anchored bait protein and solubly expressed, epitope-tagged prey protein. Upon disruption of the outer membrane, only prey proteins that bind to the bait remain cell-associated and are detected by flow cytometry using fluorescently labeled anti-epitope antibodies. In the second part of this work we developed a new strategy to engineer scFv that can be expressed in soluble and active form in the absence of disulfide bonds. This was achieved using a strain incapable of forming disulfide bonds in proteins expressed in its periplasm in combination with the APEx 2-hybrid system. The selected clones exhibited higher solubility, activity, and stability than that of the wild type scFv in the reducing condition of the cytoplasm. Finally, we sought to isolate E. coli gene fragments that can enhance IgG production in the periplasm of E. coli by a newly developed screening system based on soluble expression of IgG and E. coli genomic fragments. The isolated gene fragments, which are located between moeA and iaaA in the E. coli chromosome, improved the total expression of polypeptides of IgG and also assembly of IgG. === text
author Seo, Min Jeong, 1979-
author_facet Seo, Min Jeong, 1979-
author_sort Seo, Min Jeong, 1979-
title Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli
title_short Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli
title_full Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli
title_fullStr Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli
title_full_unstemmed Development of high throughput screening systems for the efficient production of antibody fragments in Escherichia coli
title_sort development of high throughput screening systems for the efficient production of antibody fragments in escherichia coli
publishDate 2012
url http://hdl.handle.net/2152/17756
work_keys_str_mv AT seominjeong1979 developmentofhighthroughputscreeningsystemsfortheefficientproductionofantibodyfragmentsinescherichiacoli
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