2018
DOI: 10.1021/acs.jpcb.8b09829
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Crowding Effects on Energy-Transfer Efficiencies of Hetero-FRET Probes As Measured Using Time-Resolved Fluorescence Anisotropy

Abstract: Macromolecular crowding is prevalent in all living cells due to the presence of large biomolecules and organelles. Cellular crowding is heterogeneous and is known to influence biomolecular transport, biochemical reactions, and protein folding. Emerging evidence suggests that some cell pathologies may be correlated with compartmentalized crowding. As a result, there is a need for robust biosensors that are sensitive to crowding as well as quantitative, noninvasive fluorescence methods that are compatible with l… Show more

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Cited by 21 publications
(38 citation statements)
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“…When excited at 425 nm, the time-resolved fluorescence, F ( t ), of the donor (475/50 nm) in the intact RD, KE, and RE constructs is satisfactorily described as a biexponential decay model such that In this model, we assume that α 1 and α 2 are amplitude fractions (α 1 + α 2 = 1) of two distinct subpopulations; one undergoes FRET (at a rate of k ET + k fl D and amplitude α 1 ) and the other population decays only via fluorescence (i.e., no FRET) at a rate of k fl D and amplitude α 2 . The biexponential decay model was satisfactory following the Akaike information criterion .…”
Section: Discussionmentioning
confidence: 99%
“…When excited at 425 nm, the time-resolved fluorescence, F ( t ), of the donor (475/50 nm) in the intact RD, KE, and RE constructs is satisfactorily described as a biexponential decay model such that In this model, we assume that α 1 and α 2 are amplitude fractions (α 1 + α 2 = 1) of two distinct subpopulations; one undergoes FRET (at a rate of k ET + k fl D and amplitude α 1 ) and the other population decays only via fluorescence (i.e., no FRET) at a rate of k fl D and amplitude α 2 . The biexponential decay model was satisfactory following the Akaike information criterion .…”
Section: Discussionmentioning
confidence: 99%
“…The well-separated absorption/emission bands of eGFP and mRFP1 ensured minimal donor bleed-through, which inevitably resulted in smaller spectral overlap, and, hence, less efficient FRET. The group of Heikal developed mCerulean-mCitrine-based biosensors to study macromolecular crowding in cells 44 , 45 . They used time-resolved anisotropy to analyze the rotational dynamics of the probes, but eliminating donor background and subsequent quantification of angular displacement were not in the scope of their research.…”
Section: Discussionmentioning
confidence: 99%
“…This model system was selected due to its low energy transfer efficiency (7.1 ± 0.5)% as measured using time-resolved fluorescence ( Aplin et al, 2020 ) to test the sensitivity of the proposed FCS approach. For the control experiments on the donor alone, the linker region of the FRET probe (mTurquoise2.1–link–mCitrine) was digested using the serine protease, proteinase K ( Leopold et al, 2019 ; Schwarz et al, 2019 ; Miller et al, 2020 ; Aplin et al, 2021 ) ( Figure 1B ). The absorption and emission spectra of crTC2.1 construct in a buffer are also shown ( Figure 1C ), where the excitation wavelength of the donor (405 nm) and its fluorescence detection can be visualized (arrows).…”
Section: Materials and Experimental Design Using Conventional Fcs Setupmentioning
confidence: 99%
“…In addition, FRET has been used successfully to study intermolecular interactions and their dynamics in a myriad of biological systems, both in vitro and in vivo ( Lakowicz, 2006 ; Piston and Kremers, 2007 ; Zhang et al, 2013 ; Shrestha et al, 2015 ; Okamoto and Sako, 2017 ; Schwarz et al, 2019 ; Miller et al, 2020 ). FRET applications in scientific research include molecule-molecule interactions ( Margineanu et al, 2016 ), conformational changes of biomolecules ( Ha et al, 1996 ), and environmental sensing ( Leopold et al, 2019 ; Schwarz et al, 2019 ; Miller et al, 2020 ).…”
Section: Introductionmentioning
confidence: 99%
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