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논문 기본 정보
- 자료유형
- 학술저널
- 저자정보
- 저널정보
- 한국미생물생명공학회 Journal of Microbiology and Biotechnology Journal of Microbiology and Biotechnology 제20권 제10호
- 발행연도
- 2010.1
- 수록면
- 1,463 - 1,470 (8page)
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초록· 키워드
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E. coli has long been widely used as a host system for the manufacture of recombinant proteins intended for human therapeutic use. When considering the impurities to be eliminated during the downstream process, residual host cell DNA is a major safety concern. The presence of residual E. coli host cell DNA in the final products is typically determined using a conventional slot blot hybridization assay or total DNA Threshold assay. However,both the former and latter methods are time consuming,expensive, and relatively insensitive. This study thus attempted to develop a more sensitive real-time PCR assay for the specific detection of residual E. coli DNA.
This novel method was then compared with the slot blot hybridization assay and total DNA Threshold assay in order to determine its effectiveness and overall capabilities.
The novel approach involved the selection of a specific primer pair for amplification of the E. coli 16S rRNA gene in an effort to improve sensitivity, whereas the E. coli host cell DNA quantification took place through the use of SYBR Green I. The detection limit of the real-time PCR assay, under these optimized conditions, was calculated to be 0.042 pg genomic DNA, which was much higher than those of both the slot blot hybridization assay and total DNA Threshold assay, where the detection limits were 2.42 and 3.73 pg genomic DNA, respectively. Hence, the real-time PCR assay can be said to be more reproducible,more accurate, and more precise than either the slot blot hybridization assay or total DNA Threshold assay. The real-time PCR assay may thus be a promising new tool for the quantitative detection and clearance validation of residual E. coli host cell DNA during the manufacturing process for recombinant therapeutics.
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참고문헌 (21)
참고문헌 신청
Banexy, F / 1999 / Recombinant protein expression in Escherichia coli / Curr. Opin. Biotechnol 10 : 411 ~ 421
Brosius, J / 1981 / Gene organization and primary structure of a ribosomal RNA operon from Escherichia coli / J. Bacteriol 62 : 293 ~ 300
CPMP / 1997 / Position Statement on DNA and host cell proteins (HCP) impurities - routine testing versus validation studies / Biotechnology Working Party, Committee for Proprietary Med
CPMP / 2001 / Position statement on the use of tumourigenic cells of human origin for the production of biological and biotechnological medicinal products / Biotechnology Working Party
FDA / 1997 / Points to consider in the manufacture and testing of monoclonal antibody products for human use / US Department of Health and Human Services, Food and Drug Administration,
Brosius, J / 1981 / Gene organization and primary structure of a ribosomal RNA operon from Escherichia coli / J. Bacteriol 62 : 293 ~ 300
CPMP / 1997 / Position Statement on DNA and host cell proteins (HCP) impurities - routine testing versus validation studies / Biotechnology Working Party, Committee for Proprietary Med
CPMP / 2001 / Position statement on the use of tumourigenic cells of human origin for the production of biological and biotechnological medicinal products / Biotechnology Working Party
FDA / 1997 / Points to consider in the manufacture and testing of monoclonal antibody products for human use / US Department of Health and Human Services, Food and Drug Administration,
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