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Citation
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HERO ID
6406346
Reference Type
Journal Article
Title
Peak emission wavelength and fluorescence lifetime are coupled in far-red, GFP-like fluorescent proteins
Author(s)
Canty, L; Hariharan, S; Liu, Q; Haney, SA; Andrews, DW
Year
2018
Is Peer Reviewed?
1
Journal
PLoS ONE
EISSN:
1932-6203
Volume
13
Issue
11
Page Numbers
e0208075
Language
English
PMID
30485364
DOI
10.1371/journal.pone.0208075
URL
http://dx.plos.org/10.1371/journal.pone.0208075
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Abstract
The discovery and use of fluorescent proteins revolutionized cell biology by allowing the visualization of proteins in living cells. Advances in fluorescent proteins, primarily through genetic engineering, have enabled more advanced analyses, including Förster resonance energy transfer (FRET) and fluorescence lifetime imaging microscopy (FLIM) and the development of genetically encoded fluorescent biosensors. These fluorescence protein-based sensors are highly effective in cells grown in monolayer cultures. However, it is often desirable to use more complex models including tissue explants, organoids, xenografts, and whole animals. These types of samples have poor light penetration owing to high scattering and absorption of light by tissue. Far-red light with a wavelength between 650-900nm is less prone to scatter, and absorption by tissues and can thus penetrate more deeply. Unfortunately, there are few fluorescent proteins in this region of the spectrum, and they have sub-optimal fluorescent properties including low brightness and short fluorescence lifetimes. Understanding the relationships between the amino-acid sequences of far-red fluorescence proteins and their photophysical properties including peak emission wavelengths and fluorescence lifetimes would be useful in the design of new fluorescence proteins for this region of the spectrum. We used both site-directed mutagenesis and gene-shuffling between mScarlet and mCardinal fluorescence proteins to create new variants and assess their properties systematically. We discovered that for far-red, GFP-like proteins the emission maxima and fluorescence lifetime have a strong inverse correlation.
Keywords
; Amino Acid Sequence; Fluorescence; HEK293 Cells; Humans; Luminescent Proteins/chemistry; Luminescent Proteins/genetics; Luminescent Proteins/metabolism; Microscopy; Fluorescence; Mutagenesis; Site-Directed; Spectrum Analysis; Index Medicus/
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