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      형질전환 벼 현탁세포 배양에서 hCTLA4Ig의 in situ 회수

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      https://www.riss.kr/link?id=A102592320

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      다국어 초록 (Multilingual Abstract)

      In this research, recombinant human cytotoxic Tlymphocyte antigen 4-immunoglobulin (hCTLA4Ig) was produced by transgenic rice cells. RAmy3D promoter was used for overcome the limitation of low expression level in transgenic plant cells, and the secret...

      In this research, recombinant human cytotoxic Tlymphocyte antigen 4-immunoglobulin (hCTLA4Ig) was produced by transgenic rice cells. RAmy3D promoter was used for overcome the limitation of low expression level in transgenic plant cells, and the secretion of target protein was accomplished by signal peptide. However, the RAmy3D promoter system which can be induced only by sugar starvation causes the decrease of cell viability. As a result, cell death promotes the release of protease which degrades the target proteins. The protein stability and productivity can be significantly influenced by proteolysis activity. Therefore, development of new strategies are necessary for the in situ recovery of target proteins from cell culture media. In this study, in situ recovery was performed by various strategies. Direct addition of Protein A resin with nylon bag leads to cell death by increased shear stress and decrease in production of hCTLA4Ig by protease. Medium exchange through modified flask could recover hCTLA4Ig with high cell viability and low protease activity, on the other hand, the productivity was lower than that of control. When in situ recovery was conducted at day 7 after induction in air-lift bioreactor, 1.94-fold of hCTLA4Ig could be recovered compared to control culture without in situ recovery. Consequently, in situ recovery of hCTLA4Ig from transgenic rice cell culture could enhance productivity significantly and prevent degradation of target proteins effectively.

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      목차 (Table of Contents)

      • Abstract
      • 1. INTRODUCTION
      • 2. MATERIALS AND METHODS
      • 3. RESULTS AND DISCUSSION
      • 4. CONCLUSION
      • Abstract
      • 1. INTRODUCTION
      • 2. MATERIALS AND METHODS
      • 3. RESULTS AND DISCUSSION
      • 4. CONCLUSION
      • REFERENCES
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      참고문헌 (Reference)

      1 Chakrabarti, S. K., "Purification and characterization of an extracellular alkaline serine protease from Aspergillus terreus" 40 : 239-244, 2000

      2 Toyofuku, K., "Promoter elements required for sugar-repression of the RAmy3D gene for α-amylase in rice" 428 : 275-280, 1998

      3 He, X., "Production of α-L-iduronidase in maize for the potential treatment of a human lysosomal storage disease" 3 : 1062-, 2012

      4 Jung, J. -W., "Production and characterization of recombinant human acid α-glucosidase in transgenic rice cell suspension culture" 226 : 44-53, 2016

      5 Lee, S. -J., "Production and characterization of human CTLA4Ig expressed in transgenic rice cell suspension cultures" 51 : 293-302, 2007

      6 J. F. Buyel, "Process development strategies in plant molecular farming" 16 : 966-982, 2015

      7 Kwon, J.-Y., "Process characterization of hCTLA4Ig production in transgenic rice cell cultures using a 3-L bioreactor" 171 : 1276-1288, 2013

      8 James, E., "Increased production and recovery of secreted foreign proteins from plant cell cultures using an affinity chromatography bioreactor" 12 : 205-213, 2002

      9 Stark, D., "In situ product removal (ISPR)in whole cell biotechnology during the last twenty years" 80 : 149-175, 2003

      10 Kuo, Y.-C., "Improving pharmaceutical protein production in Oryza sativa" 14 : 8719-8739, 2013

      1 Chakrabarti, S. K., "Purification and characterization of an extracellular alkaline serine protease from Aspergillus terreus" 40 : 239-244, 2000

      2 Toyofuku, K., "Promoter elements required for sugar-repression of the RAmy3D gene for α-amylase in rice" 428 : 275-280, 1998

      3 He, X., "Production of α-L-iduronidase in maize for the potential treatment of a human lysosomal storage disease" 3 : 1062-, 2012

      4 Jung, J. -W., "Production and characterization of recombinant human acid α-glucosidase in transgenic rice cell suspension culture" 226 : 44-53, 2016

      5 Lee, S. -J., "Production and characterization of human CTLA4Ig expressed in transgenic rice cell suspension cultures" 51 : 293-302, 2007

      6 J. F. Buyel, "Process development strategies in plant molecular farming" 16 : 966-982, 2015

      7 Kwon, J.-Y., "Process characterization of hCTLA4Ig production in transgenic rice cell cultures using a 3-L bioreactor" 171 : 1276-1288, 2013

      8 James, E., "Increased production and recovery of secreted foreign proteins from plant cell cultures using an affinity chromatography bioreactor" 12 : 205-213, 2002

      9 Stark, D., "In situ product removal (ISPR)in whole cell biotechnology during the last twenty years" 80 : 149-175, 2003

      10 Kuo, Y.-C., "Improving pharmaceutical protein production in Oryza sativa" 14 : 8719-8739, 2013

      11 Woodley, J. M., "Future directions for in-situ product removal" 83 : 121-123, 2008

      12 W. R. Strohl, "Fusion proteins for half-life extension of biologics as a strategy to make biobetters" 29 : 215-239, 2015

      13 Roja, G., "Enhanced production of the polysaccharide arabinogalactan using immobilized cultures of Tinospora cordifolia by elicitation and in situ adsorption" 21 : 1688-1691, 2005

      14 Komaraiah, P., "Enhanced production of plumbagin in immobilized cells of Plumbago rosea by elicitation and in situ adsorption" 101 : 181-187, 2003

      15 Kwon, J.-Y., "Application of anoxia with glucose addition for the enhanced production of hCTLA4Ig in transgenic rice suspension cell cultures" 50 : 298-303, 2012

      16 Takatsuka, C., "3-Methyladenine inhibits autophagy in tobacco culture cells under sucrose starvation conditions" 45 : 265-274, 2004

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      학술지 이력

      학술지 이력
      연월일 이력구분 이력상세 등재구분
      2022 평가예정 재인증평가 신청대상 (재인증)
      2019-01-01 평가 등재학술지 유지 (계속평가) KCI등재
      2016-01-01 평가 등재학술지 선정 (계속평가) KCI등재
      2015-12-01 평가 등재후보로 하락 (기타) KCI등재후보
      2011-01-01 평가 등재학술지 유지 (등재유지) KCI등재
      2009-08-28 학술지명변경 한글명 : 한국생물공학회지 -> KSBB Journal
      외국어명 : Korean Journal of Biotechnology and Bioengineering -> Korean Society for Biotechnology and Bioengineering Journal
      KCI등재
      2009-01-01 평가 등재학술지 유지 (등재유지) KCI등재
      2007-01-01 평가 등재학술지 유지 (등재유지) KCI등재
      2005-01-01 평가 등재학술지 유지 (등재유지) KCI등재
      2002-01-01 평가 등재학술지 선정 (등재후보2차) KCI등재
      1999-07-01 평가 등재후보학술지 선정 (신규평가) KCI등재후보
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      학술지 인용정보

      학술지 인용정보
      기준연도 WOS-KCI 통합IF(2년) KCIF(2년) KCIF(3년)
      2016 0.37 0.37 0.38
      KCIF(4년) KCIF(5년) 중심성지수(3년) 즉시성지수
      0.37 0.36 0.662 0.02
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