Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody

The project serves to identify a suitable prokaryotic expression system and protocol for routine production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) clone B10 antibody. The antibody product is meant to bind to EGFRs and has diagnostic and potential therapeutic a...

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Main Author: Loh, Valerie Kai Li.
Other Authors: Lim Sierin
Format: Final Year Project
Language:English
Published: 2011
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Online Access:http://hdl.handle.net/10356/45746
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Institution: Nanyang Technological University
Language: English
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spelling sg-ntu-dr.10356-457462023-03-03T15:40:57Z Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody Loh, Valerie Kai Li. Lim Sierin School of Chemical and Biomedical Engineering DRNTU::Engineering::Chemical engineering::Biotechnology The project serves to identify a suitable prokaryotic expression system and protocol for routine production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) clone B10 antibody. The antibody product is meant to bind to EGFRs and has diagnostic and potential therapeutic applications, for instance, conjugating to a carrier for drug delivery purposes. Initially, optimization of yield was attempted via use of different induction strategies, coupled with the use of various expression systems, including the use of commercially available pET vectors and BL21 host strain derivatives that have been well-published. Subsequently, the scFv-EGFR B10 gene sequence underwent codon optimization and a different expression system, pSYN1 vector and E. coli TG1 competent host strain, was used. Affinity chromatography and size-exclusion chromatography via Fast Protein Liquid Chromatography (FPLC) are the methods of purification and protein products are characterised using sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and/or Western blot. Results show that the antibody product may not have been produced successfully using the initial expression system due to recurring inconclusive results from purification and characterisation procedures. However, with the use of pSYN1/TG1 expression system and protocol, Western blot results appear to show positive production of scFv-EGFR B10 (synthetic optimized sequence), and specific affinity of the scFv-EGFR B10 antibody product to EGFR is proven. Bachelor of Engineering (Chemical and Biomolecular Engineering) 2011-06-16T09:03:02Z 2011-06-16T09:03:02Z 2011 2011 Final Year Project (FYP) http://hdl.handle.net/10356/45746 en Nanyang Technological University 95 p. application/pdf
institution Nanyang Technological University
building NTU Library
continent Asia
country Singapore
Singapore
content_provider NTU Library
collection DR-NTU
language English
topic DRNTU::Engineering::Chemical engineering::Biotechnology
spellingShingle DRNTU::Engineering::Chemical engineering::Biotechnology
Loh, Valerie Kai Li.
Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody
description The project serves to identify a suitable prokaryotic expression system and protocol for routine production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) clone B10 antibody. The antibody product is meant to bind to EGFRs and has diagnostic and potential therapeutic applications, for instance, conjugating to a carrier for drug delivery purposes. Initially, optimization of yield was attempted via use of different induction strategies, coupled with the use of various expression systems, including the use of commercially available pET vectors and BL21 host strain derivatives that have been well-published. Subsequently, the scFv-EGFR B10 gene sequence underwent codon optimization and a different expression system, pSYN1 vector and E. coli TG1 competent host strain, was used. Affinity chromatography and size-exclusion chromatography via Fast Protein Liquid Chromatography (FPLC) are the methods of purification and protein products are characterised using sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and/or Western blot. Results show that the antibody product may not have been produced successfully using the initial expression system due to recurring inconclusive results from purification and characterisation procedures. However, with the use of pSYN1/TG1 expression system and protocol, Western blot results appear to show positive production of scFv-EGFR B10 (synthetic optimized sequence), and specific affinity of the scFv-EGFR B10 antibody product to EGFR is proven.
author2 Lim Sierin
author_facet Lim Sierin
Loh, Valerie Kai Li.
format Final Year Project
author Loh, Valerie Kai Li.
author_sort Loh, Valerie Kai Li.
title Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody
title_short Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody
title_full Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody
title_fullStr Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody
title_full_unstemmed Production of single-chain variable fragment epidermal growth factor receptor (scFv-EGFR) antibody
title_sort production of single-chain variable fragment epidermal growth factor receptor (scfv-egfr) antibody
publishDate 2011
url http://hdl.handle.net/10356/45746
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