4.8 Article

Enhancement of Aggregation-Induced Emission in Dye-Encapsulating Polymeric Micelles for Bioimaging

期刊

ADVANCED FUNCTIONAL MATERIALS
卷 20, 期 9, 页码 1413-1423

出版社

WILEY-V C H VERLAG GMBH
DOI: 10.1002/adfm.200902043

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资金

  1. Microscale Life Sciences Center (MLSC)
  2. NIH
  3. National Science Foundation's NSF-STC [DMR-0120967]
  4. National Research Foundation of Korea under the Ministry of Education, Science and Technology [R31-10035]
  5. National Science Council of Taiwan [NSC-096-2917-1-564-115]
  6. Ministry of Education, Science & Technology (MoST), Republic of Korea [R31-2008-000-10035-0] Funding Source: Korea Institute of Science & Technology Information (KISTI), National Science & Technology Information Service (NTIS)

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Three amphiphilic block copolymers are employed to form polymeric micelles and function as nanocarriers to disperse hydrophobic aggregation-induced emission (AIE) dyes, 1,1,2,3,4,5-hexaphenylsilole (HPS) and/or bis(4-(N-(1-naphthyl) phenylamino)-phenyl)fumaronitrile (NPAFN), into aqueous solution for biological studies. Compared to their virtually non-emissive properties in organic solutions, the fluorescence intensity of these AIE dyes has increased significantly due to the spatial confinement that restricts intramolecular rotation of these dyes and their better compatibility in the hydrophobic core of polymeric micelles. The effect of the chemical structure of micelle cores on the photophysical properties of AIE dyes are investigated, and the fluorescence resonance energy transfer (FRET) from the green-emitting donor (HPS) to the red-emitting acceptor (NPAFN) is explored by co-encapsulating this FRET pair in the same micelle core. The highest fluorescence quantum yield (similar to 62%) could be achieved by encapsulating H PS aggregates in the micelles. Efficient energy transfer (>99%) and high amplification of emission (as high as 8 times) from the NPAFN acceptor could also be achieved by spatially confining the HPS/NPAFN FRET pair in the hydrophobic core of polymeric micelles. These micelles could be successfully internalized into the RAW 264.7 cells to demonstrate high-quality fluorescent images and cell viability due to improved quantum yield and reduced cytotoxicity.

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