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Please use this identifier to cite or link to this item: https://doi.org/10.1038/ncomms11964
Title: Development of background-free tame fluorescent probes for intracellular live cell imaging
Authors: Alamudi, S.H 
Satapathy, R 
Kim, J
Su, D
Ren, H
Das, R 
Hu, L
Alvarado-Martínez, E
Lee, J.Y 
Hoppmann, C
Penã-Cabrera, E
Ha, H.-H
Park, H.-S
Wang, L
Chang, Y.-T 
Keywords: alpha tubulin
fluorescent dye
4,4-difluoro-4-bora-3a,4a-diaza-s-indacene
azide
boron derivative
cyclooctane derivative
fluorescent dye
recombinant protein
cell organelle
cells and cell components
cellular automaton
fluorescence
permeability
protein
solubility
animal cell
Article
cell function
cell membrane
cell membrane permeability
cell organelle
cell proliferation
controlled study
fluorescence
genetic transfection
high throughput screening
imaging
in vitro study
lipophilicity
live cell imaging
nonhuman
quantitative structure activity relation
reliability
solubility
surface area
Western blotting
animal
chemistry
CHO cell line
Cricetulus
drug design
gene expression
genetics
Golgi complex
human
lysosome
metabolism
mitochondrion
molecular imaging
nucleolus
osteoblast
procedures
signal noise ratio
staining
synthesis
tumor cell line
ultrastructure
Animals
Azides
Boron Compounds
Cell Line, Tumor
Cell Nucleolus
CHO Cells
Cricetulus
Cyclooctanes
Drug Design
Fluorescent Dyes
Gene Expression
Golgi Apparatus
High-Throughput Screening Assays
Humans
Lysosomes
Mitochondria
Molecular Imaging
Osteoblasts
Recombinant Proteins
Signal-To-Noise Ratio
Staining and Labeling
Issue Date: 2016
Publisher: Nature Publishing Group
Citation: Alamudi, S.H, Satapathy, R, Kim, J, Su, D, Ren, H, Das, R, Hu, L, Alvarado-Martínez, E, Lee, J.Y, Hoppmann, C, Penã-Cabrera, E, Ha, H.-H, Park, H.-S, Wang, L, Chang, Y.-T (2016). Development of background-free tame fluorescent probes for intracellular live cell imaging. Nature Communications 7 : 11964. ScholarBank@NUS Repository. https://doi.org/10.1038/ncomms11964
Abstract: Fluorescence labelling of an intracellular biomolecule in native living cells is a powerful strategy to achieve in-depth understanding of the biomolecule's roles and functions. Besides being nontoxic and specific, desirable labelling probes should be highly cell permeable without nonspecific interactions with other cellular components to warrant high signal-to-noise ratio. While it is critical, rational design for such probes is tricky. Here we report the first predictive model for cell permeable background-free probe development through optimized lipophilicity, water solubility and charged van der Waals surface area. The model was developed by utilizing high-throughput screening in combination with cheminformatics. We demonstrate its reliability by developing CO-1 and AzG-1, a cyclooctyne-and azide-containing BODIPY probe, respectively, which specifically label intracellular target organelles and engineered proteins with minimum background. The results provide an efficient strategy for development of background-free probes, referred to as 'tame' probes, and novel tools for live cell intracellular imaging.
Source Title: Nature Communications
URI: https://scholarbank.nus.edu.sg/handle/10635/174954
ISSN: 20411723
DOI: 10.1038/ncomms11964
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