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KCIMicroencapsulation of cells within microfluidic devices enables explicit control of the membrane thickness or cell density, resulting in improved viability of the transplanted cells within an aggressive immune system. In this study, living cells (3T3 ...
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RISS 인기검색어
https://www.riss.kr/link?id=A104426823
-
저자
Justin Cooper-White (The University of Queensland) ; Joung Sook Hong (고려대학교) ; 신수정 (고려대학교) ; 이상훈 (고려대학교) ; Edeline Wong (The University of Queensland)
- 발행기관
- 학술지명
- 권호사항
-
발행연도
2007
-
작성언어
-
-
주제어
calcium alginate gel ; bead ; fibre ; microencapsulation ; microfluidics1. IntroductionImmune protection of cells using encapsulation technology has been proposed as a notable method to improve cellular viability following transplantation (Chang ; 1964). ; calcium alginate gel ; bead ; fibre ; microencapsulation ; microfluidics1. IntroductionImmune protection of cells using encapsulation technology has been proposed as a notable method to improve cellular viability following transplantation (Chang ; 1964).
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등재정보
KCI등재후보,SCIE,SCOPUS
-
자료형태
학술저널
-
수록면
157-164(8쪽)
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KCI 피인용횟수
8
- 제공처
-
0
상세조회 -
0
다운로드
부가정보
다국어 초록 (Multilingual Abstract)
Microencapsulation of cells within microfluidic devices enables explicit control of the membrane thickness or cell density, resulting in improved viability of the transplanted cells within an aggressive immune system. In this study, living cells (3T3 and L929 fibroblast cells) are encapsulated within a semi-permeable membrane (calcium crosslinked alginate gel) in two different device designs, a flow focusing and a core-annular flow focusing geometry. These two device designs produce a bead and a long microfibre, respectively. For the alginate bead, an alginate aqueous solution incorporating cells flows through a flow focusing channel and an alginate droplet is formed from the balance of interfacial forces and viscous drag forces resulting from the continuous (oil) phase flowing past the alginate solution. It immediately reacts with an adjacent CaCl2 drop that is extruded into the main flow channel by another flow focusing channel downstream of the site of alginate drop creation. Depending on the flow conditions, monodisperse microbeads of sizes ranging from 50-200 m can be produced. In the case of the microfibre, the alginate solution with cells is extruded into a continuous phase of CaCl2 solution. The diameter of alginate fibres produced via this technique can be tightly controlled by changing both flow rates. Cell viability in both forms of alginate encapsulant was confirmed by a LIVE/DEAD cell assay for periods of up to 24 hours post encapsulation.
참고문헌 (Reference)
1 "au 2007 by The Korean Society of Rheology"
2 "au 2007 by The Korean Society of Rheology"
3 "The generation of highly monodisperse droplets through the breakup of hydrodynamically focused microthread in a microfluidic device" 85 (85): 3726-3728, 2004
4 "Size control of calcium alginate beads containing living cells using micro-nozzle array" 26 : 3327-3331, 2005
5 "Poly-L-lysine induces fibrosis on alginate microcapsules via the induction of cytokines" 10 : 263-275, 2001
6 "Pluronic F127 as a cell encapsulation material: utilization of membrane-stabilizing agents" 11 (11): 974-983, 2005
7 "On the capillary phenomena of jets" 71-97, 1879
8 "Normalization of diabetes in spontaneously diabetic cynomologous monkeys by xenografts of microencapsulated porcine islets without immunosuppression" 98 : 1417-1422, 1996
9 "Monodisperse double emulsions generated from a microcapillary device" 308 : 537-541, 2005
10 "Microfluidic Lab-on a-chip for chemical and biological analysis and discovery" CRC press 2006
1 "au 2007 by The Korean Society of Rheology"
2 "au 2007 by The Korean Society of Rheology"
3 "The generation of highly monodisperse droplets through the breakup of hydrodynamically focused microthread in a microfluidic device" 85 (85): 3726-3728, 2004
4 "Size control of calcium alginate beads containing living cells using micro-nozzle array" 26 : 3327-3331, 2005
5 "Poly-L-lysine induces fibrosis on alginate microcapsules via the induction of cytokines" 10 : 263-275, 2001
6 "Pluronic F127 as a cell encapsulation material: utilization of membrane-stabilizing agents" 11 (11): 974-983, 2005
7 "On the capillary phenomena of jets" 71-97, 1879
8 "Normalization of diabetes in spontaneously diabetic cynomologous monkeys by xenografts of microencapsulated porcine islets without immunosuppression" 98 : 1417-1422, 1996
9 "Monodisperse double emulsions generated from a microcapillary device" 308 : 537-541, 2005
10 "Microfluidic Lab-on a-chip for chemical and biological analysis and discovery" CRC press 2006
11 "Microencapsulated islets as bioartificial endocrine pancreas" 908-210 910, 1980
12 "Method for the isolation of intact islets of Langerhans from the rat pancreas" kostia (kostia): 35-16 39, 1967
13 "Formation of dispersions using "flow focusing" in microchannels" 82 (82): 364-366, 2003
14 "Drop formation of a non-Newtonian fluid in a flow-focusing microfluidic channel" 2007
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분석정보
인용정보 인용지수 설명보기
학술지 이력
| 연월일 | 이력구분 | 이력상세 | 등재구분 |
|---|---|---|---|
| 2023 | 평가예정 | 해외DB학술지평가 신청대상 (해외등재 학술지 평가) | |
| 2020-01-01 | 평가 | 등재학술지 유지 (해외등재 학술지 평가) |  |
| 2012-01-01 | 평가 | SCIE 등재 (등재유지) | |
| 2012-01-01 | 평가 | SCOPUS 등재 (등재유지) | |
| 2011-01-01 | 평가 | 등재후보학술지 유지 (등재후보2차) |  |
| 2010-01-01 | 평가 | 등재후보 1차 PASS (등재후보1차) | |
| 2003-01-01 | 평가 | SCIE 등재 (신규평가) | |
학술지 인용정보
| 기준연도 | WOS-KCI 통합IF(2년) | KCIF(2년) | KCIF(3년) |
|---|---|---|---|
| 2016 | 1.01 | 0.18 | 0.77 |
| KCIF(4년) | KCIF(5년) | 중심성지수(3년) | 즉시성지수 |
| 0.59 | 0.52 | 0.327 | 0.06 |
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