automation;
bioprocess;
human papillomavirus;
microscale;
chromatography;
fermentation;
virus-like particle (VLP);
D O I:
10.1042/BA20060240
中图分类号:
Q5 [生物化学];
Q7 [分子生物学];
学科分类号:
071010 ;
081704 ;
摘要:
The development of fermentation processes for recombinant vaccines requires optimizing expression while maintaining high product quality. Changes to cell fermentation conditions are typically evaluated following cell disruption, with expression levels quantified by immunoassay, liquid chromatography or enzyme activity. However, assay titres do not always predict the effects that intracellular aggregation, proteolysis, posttranslational modifications and differences in relative impurity levels can have on purification yield and product purity. Furthermore, heterogeneity in the size and surface properties inherent in viral particles makes unit operations such as chromatography less predictable. In these cases, the purification procedure (or a mimic thereof) must be carried out to give accurate information on the impact of changes in fermentation conditions on purification process performance. This was demonstrated for the development of a recombinant vaccine against human papillomavirus produced in Soccharomyces cerevisiae, where the most informative feedback on fermentation variables was obtained by completing a multistep chromatographic purification to evaluate process yield and product purity. To increase the purification throughput and reduce labour, the chromatography was miniaturized 1000-fold from the laboratory scale using microlitre volumes of adsorbent in a pipette tip and automated on a robotic workstation. The microscale purification is shown to be predictive of the laboratory-scale purification in terms of yield and purity, while providing over a 10-fold increase in throughput and allowing for increased monitoring of fermentation processes. In addition, by reducing the volume of cells needed for this assessment, the fermentation can be correspondingly reduced in scale and carried out in parallel for additional throughput gains.
机构:
Chinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R China
Univ Chinese Acad Sci, Beijing 100049, Peoples R ChinaChinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R China
Na, Xiangming
Zhou, Weiqing
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机构:
Chinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R ChinaChinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R China
Zhou, Weiqing
Li, Juan
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机构:
Chinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R ChinaChinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R China
Li, Juan
Su, Zhiguo
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机构:
Chinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R ChinaChinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R China
Su, Zhiguo
Ma, Guanghui
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机构:
Chinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R ChinaChinese Acad Sci, Inst Proc Engn, State Key Lab Biochem Engn, Beijing 100190, Peoples R China
机构:
Shizuoka Univ, Grad Sch Sci & Technol, Dept Biosci, Suruga Ku, 836 Ohya, Shizuoka 4228529, JapanShizuoka Univ, Grad Sch Sci & Technol, Dept Biosci, Suruga Ku, 836 Ohya, Shizuoka 4228529, Japan
Minkner, Robert
Park, Enoch Y.
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机构:
Shizuoka Univ, Res Inst Green Sci & Technol, Green Chem Res Div, Biotechnol Lab,Suruga Ku, 836 Ohya, Shizuoka 4228529, JapanShizuoka Univ, Grad Sch Sci & Technol, Dept Biosci, Suruga Ku, 836 Ohya, Shizuoka 4228529, Japan
机构:
UJF, Therex, TIMC IMAG, CNRS UMR 5525, La Tronche, France
Polish Acad Sci, Inst Biochem & Biophys, Warsaw, PolandUJF, Therex, TIMC IMAG, CNRS UMR 5525, La Tronche, France
Chroboczek, Jadwiga
Szurgot, Inga
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Polish Acad Sci, Inst Biochem & Biophys, Warsaw, PolandUJF, Therex, TIMC IMAG, CNRS UMR 5525, La Tronche, France