Fabrication of chromatographic membrane via surface-grafted membrane for protein separation

Fabrication of chromatographic membrane via surface-grafted membrane for protein separation

Chromatography process was used extensively for protein separation in biotechnology industry. Chromatography resin bead was normally packed in cylindered column during the operation. However there were limitation on using packed bed chromatography such as high pressure drop, low processing rate and...

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Main Author: Nurul Izwanie, Rasli
Format: Thesis
Language:English
English
English
Published: 2015
Subjects:
TP Chemical technology
Online Access:http://umpir.ump.edu.my/id/eprint/12586/
http://umpir.ump.edu.my/id/eprint/12586/
http://umpir.ump.edu.my/id/eprint/12586/1/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20-CD%209684.pdf
http://umpir.ump.edu.my/id/eprint/12586/2/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20-%20CD%209684%20-%20CHAP%201.pdf
http://umpir.ump.edu.my/id/eprint/12586/3/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20CD%209684%20-%20CHAP%203.pdf
id ump-12586
recordtype eprints
spelling ump-125862016-04-04T04:08:46Z http://umpir.ump.edu.my/id/eprint/12586/ Fabrication of chromatographic membrane via surface-grafted membrane for protein separation Nurul Izwanie, Rasli TP Chemical technology Chromatography process was used extensively for protein separation in biotechnology industry. Chromatography resin bead was normally packed in cylindered column during the operation. However there were limitation on using packed bed chromatography such as high pressure drop, low processing rate and slow binding. Membrane chromatography has ability to overcome the limitation of the conventional packed bed chromatography for protein separation. Membrane chromatography used an adsorptive membrane that carried specific chromatography functionality. In the current study, commercial polyamide (PA) microfiltration membrane was modified with acrylic acid monomer to prepare a membrane chromatography. Two modification methods were compared which are ultra violet (UV) photo grafting and chemical grafting via redox reaction. Modification parameters were studied using One Factor at Time (OFAT) which are initiator concentration (1-50 mM), monomer concentration (0.2-5 M) and grafting time (5-60 minutes). The best grafting technique which gave the highest protein binding capacity was achieved by using UV photo grafting. The highest lysozyme (LZY) binding capacity achieved was 0.175 mg LZY/cm2 membrane for the membrane prepared via UV photo grafting using 10 mM of benzophenone (BP) photo-initiator, 0.1 M of acrylic acid (AA) and 15 minutes of reaction time. The best conditions of UV photo grafting modification obtained from OFAT study were used in Response Surface Methodology (RSM) for optimization of protein binding. Based on the analysis of variance (ANOVA), the quadratic model was chosen with the R squared of the model was 0.9468. The optimum value for each parameter studied in RSM was 20.71 mM of BP, 0.29 M of AA and 18.19 min of grafting time. The optimized membrane chromatography was tested and characterized in term of degree of grafting, contact angle measurement, Scanning Electron Microscope (SEM), Fourier Transform Infra-Red (FTIR), pure water flux and permeability test. The protein binding capacity at optimized condition was 0.180 mg LZY/cm2. This value is less than 4% of the value predicted by the model. This quadratic model can be used successfully to produce the membrane chromatography from PA membrane through UV grafting for LZY binding. 2015-11 Thesis NonPeerReviewed application/pdf en http://umpir.ump.edu.my/id/eprint/12586/1/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20-CD%209684.pdf application/pdf en http://umpir.ump.edu.my/id/eprint/12586/2/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20-%20CD%209684%20-%20CHAP%201.pdf application/pdf en http://umpir.ump.edu.my/id/eprint/12586/3/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20CD%209684%20-%20CHAP%203.pdf Nurul Izwanie, Rasli (2015) Fabrication of chromatographic membrane via surface-grafted membrane for protein separation. Masters thesis, Universiti Malaysia Pahang. http://iportal.ump.edu.my/lib/item?id=chamo:93877&theme=UMP2
repository_type Digital Repository
institution_category Local University
institution Universiti Malaysia Pahang
building UMP Institutional Repository
collection Online Access
language English
English
English
topic TP Chemical technology
spellingShingle TP Chemical technology
Nurul Izwanie, Rasli
Fabrication of chromatographic membrane via surface-grafted membrane for protein separation
description Chromatography process was used extensively for protein separation in biotechnology industry. Chromatography resin bead was normally packed in cylindered column during the operation. However there were limitation on using packed bed chromatography such as high pressure drop, low processing rate and slow binding. Membrane chromatography has ability to overcome the limitation of the conventional packed bed chromatography for protein separation. Membrane chromatography used an adsorptive membrane that carried specific chromatography functionality. In the current study, commercial polyamide (PA) microfiltration membrane was modified with acrylic acid monomer to prepare a membrane chromatography. Two modification methods were compared which are ultra violet (UV) photo grafting and chemical grafting via redox reaction. Modification parameters were studied using One Factor at Time (OFAT) which are initiator concentration (1-50 mM), monomer concentration (0.2-5 M) and grafting time (5-60 minutes). The best grafting technique which gave the highest protein binding capacity was achieved by using UV photo grafting. The highest lysozyme (LZY) binding capacity achieved was 0.175 mg LZY/cm2 membrane for the membrane prepared via UV photo grafting using 10 mM of benzophenone (BP) photo-initiator, 0.1 M of acrylic acid (AA) and 15 minutes of reaction time. The best conditions of UV photo grafting modification obtained from OFAT study were used in Response Surface Methodology (RSM) for optimization of protein binding. Based on the analysis of variance (ANOVA), the quadratic model was chosen with the R squared of the model was 0.9468. The optimum value for each parameter studied in RSM was 20.71 mM of BP, 0.29 M of AA and 18.19 min of grafting time. The optimized membrane chromatography was tested and characterized in term of degree of grafting, contact angle measurement, Scanning Electron Microscope (SEM), Fourier Transform Infra-Red (FTIR), pure water flux and permeability test. The protein binding capacity at optimized condition was 0.180 mg LZY/cm2. This value is less than 4% of the value predicted by the model. This quadratic model can be used successfully to produce the membrane chromatography from PA membrane through UV grafting for LZY binding.
format Thesis
author Nurul Izwanie, Rasli
author_facet Nurul Izwanie, Rasli
author_sort Nurul Izwanie, Rasli
title Fabrication of chromatographic membrane via surface-grafted membrane for protein separation
title_short Fabrication of chromatographic membrane via surface-grafted membrane for protein separation
title_full Fabrication of chromatographic membrane via surface-grafted membrane for protein separation
title_fullStr Fabrication of chromatographic membrane via surface-grafted membrane for protein separation
title_full_unstemmed Fabrication of chromatographic membrane via surface-grafted membrane for protein separation
title_sort fabrication of chromatographic membrane via surface-grafted membrane for protein separation
publishDate 2015
url http://umpir.ump.edu.my/id/eprint/12586/
http://umpir.ump.edu.my/id/eprint/12586/
http://umpir.ump.edu.my/id/eprint/12586/1/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20-CD%209684.pdf
http://umpir.ump.edu.my/id/eprint/12586/2/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20-%20CD%209684%20-%20CHAP%201.pdf
http://umpir.ump.edu.my/id/eprint/12586/3/FKKSA%20-%20NURUL%20IZWANIE%20BINTI%20RASLI%20CD%209684%20-%20CHAP%203.pdf
first_indexed 2023-09-18T22:14:23Z
last_indexed 2023-09-18T22:14:23Z
_version_ 1777415239420084224

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