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Success in the bottom‐up assembly of synthetic cells will depend on strategies for the division of protocellular compartments. Here, we describe the controlled division of phase‐separated giant unilamellar lipid vesicles (GUVs). We derive an analy...
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RISS 인기검색어
https://www.riss.kr/link?id=O106430094
- 저자
- 발행기관
- 학술지명
- 권호사항
-
발행연도
2021년
-
작성언어
eng
-
Print ISSN
1433-7851
-
Online ISSN
1521-3773
-
등재정보
SCI;SCIE;SCOPUS
-
자료형태
학술저널
-
원정보자원
Angewandte Chemie international edition
-
수록면
10661-10669 [※수록면이 p5 이하이면, Review, Columns, Editor's Note, Abstract 등일 경우가 있습니다.]
-
구독기관
- 전북대학교 중앙도서관
- 성균관대학교 중앙학술정보관
- 부산대학교 중앙도서관
- 전남대학교 중앙도서관
- 제주대학교 중앙도서관
- 중앙대학교 서울캠퍼스 중앙도서관
- 인천대학교 학산도서관
- 숙명여자대학교 중앙도서관
- 서강대학교 로욜라중앙도서관
- 충남대학교 중앙도서관
- 한양대학교 백남학술정보관
- 이화여자대학교 중앙도서관
- 고려대학교 도서관
- ⓒ COPYRIGHT THE BRITISH LIBRARY BOARD: ALL RIGHT RESERVED
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다국어 초록 (Multilingual Abstract)
Success in the bottom‐up assembly of synthetic cells will depend on strategies for the division of protocellular compartments. Here, we describe the controlled division of phase‐separated giant unilamellar lipid vesicles (GUVs). We derive an analytical model based on the vesicle geometry, which makes four quantitative predictions that we verify experimentally. We find that the osmolarity ratio required for division is 2
, independent of the GUV size, while asymmetric division happens at lower osmolarity ratios. Remarkably, we show that a suitable osmolarity change can be triggered by water evaporation, enzymatic decomposition of sucrose or light‐triggered uncaging of CMNB‐fluorescein. The latter provides full spatiotemporal control, such that a target GUV undergoes division whereas the surrounding GUVs remain unaffected. Finally, we grow phase‐separated vesicles from single‐phased vesicles by targeted fusion of the opposite lipid type with programmable DNA tags to enable subsequent division cycles.
We demonstrate division of phase‐separated lipid vesicles following quantitative predictions from an analytical model. The division is controlled by metabolic decomposition or light‐triggered uncaging of a fluorophore. This provides spatiotemporal control over the division of a target vesicle. We regrow phase‐separated vesicles by targeted fusion using DNA nanotechnology.
, independent of the GUV size, while asymmetric division happens at lower osmolarity ratios. Remarkably, we show that a suitable osmolarity change can be triggered by water evaporation, enzymatic decomposition of sucrose or light‐triggered uncaging of CMNB‐fluorescein. The latter provides full spatiotemporal control, such that a target GUV undergoes division whereas the surrounding GUVs remain unaffected. Finally, we grow phase‐separated vesicles from single‐phased vesicles by targeted fusion of the opposite lipid type with programmable DNA tags to enable subsequent division cycles.
We demonstrate division of phase‐separated lipid vesicles following quantitative predictions from an analytical model. The division is controlled by metabolic decomposition or light‐triggered uncaging of a fluorophore. This provides spatiotemporal control over the division of a target vesicle. We regrow phase‐separated vesicles by targeted fusion using DNA nanotechnology.
Success in the bottom‐up assembly of synthetic cells will depend on strategies for the division of protocellular compartments. Here, we describe the controlled division of phase‐separated giant unilamellar lipid vesicles (GUVs). We derive an analytical model based on the vesicle geometry, which makes four quantitative predictions that we verify experimentally. We find that the osmolarity ratio required for division is 2
, independent of the GUV size, while asymmetric division happens at lower osmolarity ratios. Remarkably, we show that a suitable osmolarity change can be triggered by water evaporation, enzymatic decomposition of sucrose or light‐triggered uncaging of CMNB‐fluorescein. The latter provides full spatiotemporal control, such that a target GUV undergoes division whereas the surrounding GUVs remain unaffected. Finally, we grow phase‐separated vesicles from single‐phased vesicles by targeted fusion of the opposite lipid type with programmable DNA tags to enable subsequent division cycles.
We demonstrate division of phase‐separated lipid vesicles following quantitative predictions from an analytical model. The division is controlled by metabolic decomposition or light‐triggered uncaging of a fluorophore. This provides spatiotemporal control over the division of a target vesicle. We regrow phase‐separated vesicles by targeted fusion using DNA nanotechnology.
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