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Highly Efficient Aggregation-Induced Red-Emissive Organic Thermally Activated Delayed Fluorescence Materials with Prolonged Fluorescence Lifetime for Time-Resolved Luminescence Bioimaging

Authors
Qi, SujieKim, SanginNguyen, Van-NghiaKim, YoungmeeNiu, GuangleKim, GyoungmiKim, Sung-JinPark, SungnamYoon, Juyoung
Issue Date
18-Nov-2020
Publisher
AMER CHEMICAL SOC
Keywords
thermally activated delayed fluorescence (TADF); aggregation-induced emission; red emission; fluorescence imaging; time-resolved luminescence imaging
Citation
ACS APPLIED MATERIALS & INTERFACES, v.12, no.46, pp.51293 - 51301
Indexed
SCIE
SCOPUS
Journal Title
ACS APPLIED MATERIALS & INTERFACES
Volume
12
Number
46
Start Page
51293
End Page
51301
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/51482
DOI
10.1021/acsami.0c15936
ISSN
1944-8244
Abstract
Organic thermally activated delayed fluorescence (TADF) materials are emerging as potential candidates for time-resolved fluorescence imaging in biological systems. However, the development of purely organic TADF materials with bright aggregated-state emissions in the red/near-infrared (NIR) region remains challenging. Here, we report three donor-acceptor-type TADF molecules as promising candidates for time-resolved fluorescence imaging, which are engineered by direct connection of electron-donating moieties (phenoxazine or phenothiazine) and an electron-acceptor 1,8-naphthalimide (NI). Theoretically and experimentally, we elucidate that three TADF materials possessed remarkably small Delta E-ST to promote the occurrence of reverse intersystem crossing (RISC). Moreover, they all exhibit aggregation-induced red emissions and long delayed fluorescence lifetimes without the influence of molecular oxygen. More importantly, these long-lived and biocompatible TADF materials, especially the phenoxazine-substituted NI fluorophores, show great potential for high-contrast fluorescence lifetime imaging in living cells. This study provides further a molecular design strategy for purely organic TADF materials and expands the versatile biological application of long-lived fluorescence research in time-resolved luminescence imaging.
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