New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield

Rabies is still a major cause of human deaths in several developing countries. According to the World Health Organization, administration of antirabies serum or antirabies immunoglobulin is recommended for patients who have experienced a category-III exposure to rabies. Improvement of antirabies imm...

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Main Authors: Sukanda Kittipongwarakarn, Andrea Hawe, Ruedeeporn Tantipolphan, Kornvika Limsuwun, Sumana Khomvilai, Satit Puttipipatkhachorn, Wim Jiskoot
Other Authors: Mahidol University
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Published: 2018
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Online Access:https://repository.li.mahidol.ac.th/handle/123456789/11548
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spelling th-mahidol.115482018-05-03T15:42:09Z New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield Sukanda Kittipongwarakarn Andrea Hawe Ruedeeporn Tantipolphan Kornvika Limsuwun Sumana Khomvilai Satit Puttipipatkhachorn Wim Jiskoot Mahidol University Leiden University Coriolis PharmaService GmbH Thai Red Cross Agency Biochemistry, Genetics and Molecular Biology Pharmacology, Toxicology and Pharmaceutics Rabies is still a major cause of human deaths in several developing countries. According to the World Health Organization, administration of antirabies serum or antirabies immunoglobulin is recommended for patients who have experienced a category-III exposure to rabies. Improvement of antirabies immunoglobulin production is required to enhance safety and efficacy of the products. In this paper, a new method to produce equine antirabies immunoglobulin F(ab′) 2 fragments from crude plasma is proposed. First, protein G affinity chromatography was used to purify IgG from equine plasma. Moreover, purification of IgG was shown to facilitate its digestion by pepsin. Compared to the direct digestion of crude plasma, a lower amount of pepsin and a shorter digestion time were required to completely digest the purified IgG to F(ab′) 2 . Complete digestion of purified IgG to F(ab′) 2 was achieved at a pepsin/IgG (w/w) ratio of 5:45 with preservation of structure and potency. Finally, purification of F(ab′) 2 was accomplished by a combination of protein A affinity chromatography and ultrafiltration with a 50-kDa nominal molecular weight cut-off membrane. The new process resulted in 68.9 ± 0.6 (%) total recovery of F(ab′) 2 and a F(ab′) 2 product of high potency. © 2011 Elsevier B.V. All rights reserved. 2018-05-03T08:02:35Z 2018-05-03T08:02:35Z 2011-06-01 Article European Journal of Pharmaceutics and Biopharmaceutics. Vol.78, No.2 (2011), 189-195 10.1016/j.ejpb.2011.02.018 09396411 2-s2.0-79955838803 https://repository.li.mahidol.ac.th/handle/123456789/11548 Mahidol University SCOPUS https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=79955838803&origin=inward
institution Mahidol University
building Mahidol University Library
continent Asia
country Thailand
Thailand
content_provider Mahidol University Library
collection Mahidol University Institutional Repository
topic Biochemistry, Genetics and Molecular Biology
Pharmacology, Toxicology and Pharmaceutics
spellingShingle Biochemistry, Genetics and Molecular Biology
Pharmacology, Toxicology and Pharmaceutics
Sukanda Kittipongwarakarn
Andrea Hawe
Ruedeeporn Tantipolphan
Kornvika Limsuwun
Sumana Khomvilai
Satit Puttipipatkhachorn
Wim Jiskoot
New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
description Rabies is still a major cause of human deaths in several developing countries. According to the World Health Organization, administration of antirabies serum or antirabies immunoglobulin is recommended for patients who have experienced a category-III exposure to rabies. Improvement of antirabies immunoglobulin production is required to enhance safety and efficacy of the products. In this paper, a new method to produce equine antirabies immunoglobulin F(ab′) 2 fragments from crude plasma is proposed. First, protein G affinity chromatography was used to purify IgG from equine plasma. Moreover, purification of IgG was shown to facilitate its digestion by pepsin. Compared to the direct digestion of crude plasma, a lower amount of pepsin and a shorter digestion time were required to completely digest the purified IgG to F(ab′) 2 . Complete digestion of purified IgG to F(ab′) 2 was achieved at a pepsin/IgG (w/w) ratio of 5:45 with preservation of structure and potency. Finally, purification of F(ab′) 2 was accomplished by a combination of protein A affinity chromatography and ultrafiltration with a 50-kDa nominal molecular weight cut-off membrane. The new process resulted in 68.9 ± 0.6 (%) total recovery of F(ab′) 2 and a F(ab′) 2 product of high potency. © 2011 Elsevier B.V. All rights reserved.
author2 Mahidol University
author_facet Mahidol University
Sukanda Kittipongwarakarn
Andrea Hawe
Ruedeeporn Tantipolphan
Kornvika Limsuwun
Sumana Khomvilai
Satit Puttipipatkhachorn
Wim Jiskoot
format Article
author Sukanda Kittipongwarakarn
Andrea Hawe
Ruedeeporn Tantipolphan
Kornvika Limsuwun
Sumana Khomvilai
Satit Puttipipatkhachorn
Wim Jiskoot
author_sort Sukanda Kittipongwarakarn
title New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
title_short New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
title_full New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
title_fullStr New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
title_full_unstemmed New method to produce equine antirabies immunoglobulin F(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
title_sort new method to produce equine antirabies immunoglobulin f(ab′)<inf>2</inf>fragments from crude plasma in high quality and yield
publishDate 2018
url https://repository.li.mahidol.ac.th/handle/123456789/11548
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