Microbiology and Biotechnology Letters (한국미생물·생명공학회지)

The Korean Society for Microbiology and Biotechnology (한국미생물·생명공학회)
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Evaluation of Viral Inactivation Efficacy of a Continuous Flow Ultraviolet-C Reactor (UVivatec)

연속 유동 Ultraviolet-C 반응기(UVivatec)의 바이러스 불활화 효과 평가

  • Bae, Jung-Eun (Department of Biological Sciences and Center for Biopharmaceuticals Safety Validation, Hannam University) ;
  • Jeong, Eun-Kyo (Department of Biological Sciences and Center for Biopharmaceuticals Safety Validation, Hannam University) ;
  • Lee, Jae-Il (Department of Biological Sciences and Center for Biopharmaceuticals Safety Validation, Hannam University) ;
  • Lee, Jeong-Im (Department of Biological Sciences and Center for Biopharmaceuticals Safety Validation, Hannam University) ;
  • Kim, In-Seop (Department of Biological Sciences and Center for Biopharmaceuticals Safety Validation, Hannam University) ;
  • Kim, Jong-Su (College of Medicine, Pochon CHA University, and CHA Bio & Diostech)
  • 배정은 (한남대학교 생명과학과 & 바이오의약품안전성검증센터) ;
  • 정은교 (한남대학교 생명과학과 & 바이오의약품안전성검증센터) ;
  • 이재일 (한남대학교 생명과학과 & 바이오의약품안전성검증센터) ;
  • 이정임 (한남대학교 생명과학과 & 바이오의약품안전성검증센터) ;
  • 김인섭 (한남대학교 생명과학과 & 바이오의약품안전성검증센터) ;
  • 김종수 (차의과학대학교 & (주)차바이오앤디오스텍)
  • Published : 2009.12.28
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Abstract

Viral safety is an important prerequisite for clinical preparations of all biopharmaceuticals derived from plasma, cell lines, or tissues of human or animal origin. To ensure the safety, implementation of multiple viral clearance (inactivation and/or removal) steps has been highly recommended for manufacturing of biopharmaceuticals. Of the possible viral clearance strategies, Ultraviolet-C (UVC) irradiation has been known as an effective viral inactivating method. However it has been dismissed by biopharmaceutical industry as a result of the potential for protein damage and the difficulty in delivering uniform doses. Recently a continuous flow UVC reactor (UVivatec) was developed to provide highly efficient mixing and maximize virus exposure to the UV light. In order to investigate the effectiveness of UVivatec to inactivate viruses without causing significant protein damage, the feasibility of the UVC irradiation process was studied with a commercial therapeutic protein. Recovery yield in the optimized condition of $3,000\;J/m^2$ irradiation was more than 98%. The efficacy and robustness of the UVC reactor was evaluated with regard to the inactivation of human immunodeficiency virus (HIV), hepatitis A virus (HAV), bovine herpes virus (BHV), bovine viral diarrhea virus (BVDV), porcine parvovirus (PPV), bovine parvovirus (BPV), minute virus of mice (MVM), reovirus type 3 (REO), and bovine parainfluenza virus type 3 (BPIV). Non enveloped viruses (HAV, PPV, BPV, MVM, and REO) were completely inactivated to undetectable levels by $3,000\;J/m^2$ irradiation. Enveloped viruses such as HIV, BVDV, and BPIV were completely inactivated to undetectable levels. However BHV was incompletely inactivated with slight residual infectivity remaining even after $3,000\;J/m^2$ irradiation. The log reduction factors achieved by UVC irradiation were ${\geq}3.89$ for HIV, ${\geq}5.27$ for HAV, 5.29 for BHV, ${\geq}5.96$ for BVDV, ${\geq}4.37$ for PPV, ${\geq}3.55$ for BPV, ${\geq}3.51$ for MVM, ${\geq}4.20$ for REO, and ${\geq}4.15$ for BPIV. These results indicate that UVC irradiation using UVivatec was very effective and robust in inactivating all the viruses tested.

사람과 동물 유래의 혈장, 세포, 조직 등을 이용하여 생물의약품을 생산하기 위해서는 바이러스 안전성 확보가 필수적이다. 바이러스 안전성 보증을 위해 생물의약품 제조공정은 바이러스 불활화/제거 단계를 포함하여야 한다. 짧은 파장자외선(UVC) 조사는 바이러스 불활화 효과가 매우 높은 것으로 알려졌지만, UVC 조사로 인한 단백질의 변성과 대상 물질에 동일하게 조사를 할 수 있는 기계적 장치 개발의 어려움으로 인해 UVC 조사는 생물의약품 제조 공정에 사용되지 못했다. 최근에 이러한 결점을 해결한 연속 유동 UVC 반응기(UVivatec)가 개발되었다. UVivatec의 바이러스 불활화 효과 및 단백질 회수율을 검증하기 위해 단백질 의약품을 대상으로 적용가능성을 조사하였다. 최적화된 $3,000\;J/m^2$ 조사 공정에서 단백질의 회수율은 98%이상이었다. UVC 조사에 의한 human immunodeficiency virus(HIV), hepatitis A virus(HAV), bovine herpes virus(BHV), bovine viral diarrhea virus(BVDV), porcine parvovirus(PPV), bovine parvovirus(BPV), minute virus of mice(MVM), reovirus type 3(REO), bovine parainfluenza virus type 3(BPIV) 불활화 효과를 평가하였다. HAV, PPV, BPV, MVM, REO와 같은 비외피(nonenvelope) 바이러스는 $3,000\;J/m^2$ 조사량에 의해 검출한계 이하로 완벽하게 불활화되었다. HIV, BVDV, BPIV 같은 외피(envelope) 바이러스도 $3,000\;J/m^2$ 조사량에 의해 검출한계 이하로 완벽하게 불활화되었다. 또한 BHV도 매우 민감하게 불활화되었다. UVC 조사에 의한 각 바이러스들의 로그 감소율은 HIV는 ${\geq}3.89$, HAV는 ${\geq}5.27$, BHV는 5.29, BVDV는 ${\geq}5.96$, PPV는 ${\geq}4.37$, BPV는 ${\geq}3.55$, MVM은 ${\geq}3.51$, REO는 ${\geq}4.20$, BPIV는 ${\geq}4.15$이었다. 이와 같은 결과에서 UVivatec을 이용한 UVC 조사는 바이러스 불활화에 매우 효과적인 방법임을 확인하였다.

Keywords

References

  1. Adamson, S. R. 1999. Experiences of virus, retrovirus and retrovirus-like particles in chinese hamster ovary (CHO) and hybridoma cells used for production of protein therapeutics. Dev. Biol. Stand. 93: 89-96
  2. Boschetti, N., I. Niederhauser, C. Kempf, A. Stuhler, J. Lower, and J. Blumel. 2004. Different susceptibility of B19 virus and mice minute virus to low pH treatment. Transfusion 44: 1079-1086 https://doi.org/10.1111/j.1537-2995.2004.03420.x
  3. Chin, S. 1997. Virucidal treatment of blood protein products with UVC radiation. Photochem. Photobiol. 65: 423-435
  4. Choi, Y. W. and I. S. Kim. 2008. Viral clearance during the manufacture of urokinase from human urine. Biotechnol. Bioprocess Eng. 13: 25-32 https://doi.org/10.1007/s12257-007-0140-7
  5. Chudy, M., I. Budek, B. Keller-Stanislawski, K. A. McCaustland, S. Neidhold, B. H. Robertson, C. M. Nubling, R. Seitz, and J. Lower. 1999. A new cluster of hepatitis A infection in hemophiliacs traced to a contaminated plasma pool. J. Med. Virol. 57: 91-99 https://doi.org/10.1002/(SICI)1096-9071(199902)57:2<91::AID-JMV1>3.0.CO;2-L
  6. Committee for Proprietary Medicinal Products (CPMP), The European Agency for the Evaluation of Medicinal Products: Human Medicines Evaluation Unit. 1996. Note for guidance on virus validation studies: the design, contribution and interpretation of studies validating the inactivation and removal of viruses (CPMP/BWP/268/95)
  7. Garnick, R. L. 1996. Experience with viral contamination in cell culture. Dev. Biol. Stand. 88: 49-56
  8. Guertler, L. G. 2002. Virus safety of human blood, plasma, and derived products. Thromb. Res. 107: S39-S45 https://doi.org/10.1016/S0049-3848(02)00151-2
  9. Hart, H., K. Reid, and W. Hart. 1993. Inactivation of viruses during ultraviolet light treatment of human intravenous immunoglobulin and albumin. Vox Sang. 64: 82-88
  10. International Conference on Harmonisation. 1998. Guidance on viral safety evaluation of biotechnology products derived from cell lines of human or animal origin; availability. Federal Resister 63: 51074-51084
  11. Kärber, J. 1931. Beitrag zur kollectiven Behandlung pharmakologische Reihenversuche. Arch. Exp. Path. Pharmak. 162: 480-483 https://doi.org/10.1007/BF01863914
  12. Kim, I. S., Y. W. Choi, Y. Kang, H. M. Sung, and J. S. Shin. 2008. Dry-heat treatment process for enhancing viral safety of an antihemophilic factor VIII concentrate prepared from human plasma. J. Microbiol. Biotechnol. 18: 997-1003
  13. Kim, I .S., Y. W. Choi, Y. Kang, H. M. Sung, K. W. Sohn, and Y.-S. Kim. 2008. Improvement of virus safety of an antihemophilic factor IX by virus filtration process. J. Microbiol. Biotechnol. 18: 1317-1325
  14. Kleim, J. P., E. Bailly, K. E. Schneweis, H. H. Brackmann, U. Hammerstein, and P. Hanfland. 1990. Acute HIV-1 infection in patients with hemophilia treated with beta-propiolactone- UV-inactivated clotting factor. Thromb. Haemost. 64:336-337
  15. Kupfer, B., J. Oldenburg, H. H. Brackmann, B. Matz, K. E. Schneweis, and R. Kaiser. 1995. Beta-propiolactone UV inactivated clotting factor concentrate is the source of HIVinfection of 8 hemophilia B patients: confirmed. Thromb. Haemost. 74: 1386-1387
  16. Laub, R. and P. Strengers. 2002. Parvovirus and blood products. Pathol. Biol. (Paris) 50: 339-348 https://doi.org/10.1016/S0369-8114(02)00303-6
  17. Lawlor, E., S. Graham, E. Davidson, P. L. Yap, C. Cunningham, H. Daly, and I. J. Temperley. 1996. Hepatitis A transmission by factor IX concentrates. Vox Sang. 73: 189-190 https://doi.org/10.1046/j.1423-0410.1996.7120126.x
  18. Lee, D. H., H. M. Cho, H. M. Kim, J. Lee, and I. S. Jim. 2008. Real-time PCR for validation of minute virus of mice safety during the manufacture of mammalian cell culturederived biopharmaceuticals. Kor. J. Microbiol. Biotechnol. 36: 12-20
  19. Merten, O.-W. 2002. Virus contaminations of cell cultures – A biotechnological view. Cytotechnology 39: 91–116 https://doi.org/10.1023/A:1022969101804
  20. Murray, R., J. W. Oliphant, J. T. Tripp, B. Hampil, F. Ratner, and W. C. L. Diefenbach. 1955. Effect of ultraviolet radiation on the infectivity of icterogenic plasma J. Am. Med. Assoc. 157: 8-14 https://doi.org/10.1001/jama.1955.02950180010003
  21. Robinson, S. M., H. Schwinn, and A. Smith. 1992. Clotting factors and hepatitis A. Lancet 340: 1465 https://doi.org/10.1016/0140-6736(92)92652-V
  22. Rosenthal, N., F. A. Bassen, and S. R. Michael. 1950. Probable transmission of viral hepatitis by ultraviolet-irradiated plasma: report of three cases. J. Am. Med. Assoc. 144: 224-226
  23. Schmidt, S., J. Mora, S. Dolan, and J. Kauling. 2005. An integrated concept for robust and efficient virus clearance and contamination removal in biotech process. BioProcess Int. 3(September): 26-31
  24. Shin, J. S., Y. W. Choi, H. M. Sung, Y.-W. Ryu, and I. S. Kim. 2006. Enhanced virus safety of a solvent/detergenttreated antihemophilic factor IX concentrate by dry-heat treatment. Biotech. Bioprocess Eng. 11: 19-25 https://doi.org/10.1007/BF02931863
  25. Wang, A. M., S.-F. Chao, K. Remington, R. Treckmann, K. Kaiser, D. Pifat, and J. Hotta. 2004. Virus inactivation and protein recovery in a novel ultraviolet-C reactor. Vox Sang. 86: 230-238 https://doi.org/10.1111/j.0042-9007.2004.00485.x
  26. Wang, S., C. Zinderman, R. Wise, and M. Braun. 2007. Infections and human tissue transplants: review of FDA MedWatch reports 2001–2004. Cell Tissue Banking 8: 211-219 https://doi.org/10.1007/s10561-007-9034-3
  27. Wolf, A., J. Mason, W. J. Fitzpatrick, S. O. Schwartz, and S. O. Levinson. 1947. Ultraviolet irradiation of human plasma to control homologous serum jaundice. J. Am. Med. Assoc. 135: 476-477 https://doi.org/10.1001/jama.1947.02890080006003