Sorting catalytically active polymersome nanoreactors by flow cytometry
Flow cytometry is a powerful technique for high-throughput,...
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| المؤلفون الرئيسيون: | , , , , , , , |
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| مؤلفون آخرون: | |
| التنسيق: | مقال |
| اللغة: | English |
| منشور في: |
2011
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| الموضوعات: | |
| الوصول للمادة أونلاين: | https://hdl.handle.net/10356/93845 http://hdl.handle.net/10220/7282 |
| الوسوم: |
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| الملخص: | Flow cytometry is a powerful technique for high-throughput,
fluorescence-activated screening and sorting of cells (FACS).
This methodology has been extended by Griffiths to the
screening of water-in-oil microdroplets filled with an in vitro
protein expression system.[1–6] The catalytic gene product was
detected by the transformation of a co-encapsulated profluorescent
substrate into a fluorescent product. Here we
report a strategy that involves a versatile one-step preparation
procedure of enzyme filled porous and stable polymeric
capsules (polymersomes). Since the pores of the capsules are
small enough to keep enzymes in, whereas these are
sufficiently large to allow (profluorescent) substrates to enter,
enzyme activity screening can be performed by the build-up of
fluorescence, followed by FACS. To prevent the substrate
from diffusing out of the capsules, a trapping agent was added
inside the capsule. With this technology we were able to
separate enzymatically active polymersomes from non-filled
or non-active polymersomes. |
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