Crowding Effects on Energy-Transfer Efficiencies of Hetero-FRET Probes As Measured Using Time-Resolved Fluorescence Anisotropy

Leopold, Hannah; Leighton, Ryan; Schwarz, Jacob; Boersma, Arnold J.; Sheets, Erin D.; Heikal, Ahmed A.

doi:10.1021/acs.jpcb.8b09829

Cited by 21 publications

(38 citation statements)

References 76 publications

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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%

FRET Analysis of Ionic Strength Sensors in the Hofmeister Series of Salt Solutions Using Fluorescence Lifetime Measurements

Miller¹,

Aplin²,

Kay³

et al. 2020

J. Phys. Chem. B

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Living cells are complex, crowded, and dynamic and continually respond to environmental and intracellular stimuli. They also have heterogeneous ionic strength with compartmentalized variations in both intracellular concentrations and types of ions. These challenges would benefit from the development of quantitative, noninvasive approaches for mapping the heterogeneous ionic strength fluctuations in living cells. Here, we investigated a class of recently developed ionic strength sensors that consists of mCerulean3 (a cyan fluorescent protein) and mCitrine (a yellow fluorescent protein) tethered via a linker made of two charged α-helices and a flexible loop. The two helices are designed to bear opposite charges, which is hypothesized to increase the ionic screening and therefore a larger intermolecular distance. In these protein constructs, mCerulean3 and mCitrine act as a donor–acceptor pair undergoing Förster resonance energy transfer (FRET) that is dependent on both the linker amino acids and the environmental ionic strength. Using time-resolved fluorescence of the donor (mCerulean3), we determined the sensitivity of the energy transfer efficiencies and the donor–acceptor distances of these sensors at variable concentrations of the Hofmeister series of salts (KCl, LiCl, NaCl, NaBr, NaI, Na2SO4). As controls, similar measurements were carried out on the FRET-incapable, enzymatically cleaved counterparts of these sensors as well as a construct designed with two electrostatically neutral α-helices (E6G2). Our results show that the energy transfer efficiencies of these sensors are sensitive to both the linker amino acid sequence and the environmental ionic strength, whereas the sensitivity of these sensors to the identity of the dissolved ions of the Hofmeister series of salts seems limited. We also developed a theoretical framework to explain the observed trends as a function of the ionic strength in terms of the Debye screening of the electrostatic interaction between the two charged α-helices in the linker region. These controlled solution studies represent an important step toward the development of rationally designed FRET-based environmental sensors while offering different models for calculating the energy transfer efficiency using time-resolved fluorescence that is compatible with future in vivo studies.

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Section: Discussionmentioning

confidence: 99%

FRET Analysis of Ionic Strength Sensors in the Hofmeister Series of Salt Solutions Using Fluorescence Lifetime Measurements

Miller¹,

Aplin²,

Kay³

et al. 2020

J. Phys. Chem. B

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“…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%

Quantification of FRET-induced angular displacement by monitoring sensitized acceptor anisotropy using a dim fluorescent donor

Laskaratou¹,

Fernández²,

Coucke³

et al. 2021

Nat Commun

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Förster resonance energy transfer (FRET) between fluorescent proteins has become a common platform for designing genetically encoded biosensors. For live cell imaging, the acceptor-to-donor intensity ratio is most commonly used to readout FRET efficiency, which largely depends on the proximity between donor and acceptor. Here, we introduce an anisotropy-based mode of FRET detection (FADED: FRET-induced Angular Displacement Evaluation via Dim donor), which probes for relative orientation rather than proximity alteration. A key element in this technique is suppression of donor bleed-through, which allows measuring purer sensitized acceptor anisotropy. This is achieved by developing Geuda Sapphire, a low-quantum-yield FRET-competent fluorescent protein donor. As a proof of principle, Ca2+ sensors were designed using calmodulin as a sensing domain, showing sigmoidal dose response to Ca2+. By monitoring the anisotropy, a Ca2+ rise in living HeLa cells is observed upon histamine challenging. We conclude that FADED provides a method for quantifying the angular displacement via FRET.

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“…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%

“…In these constructs, the donor (mCerluean3) and acceptor (mCitrine) act as a FRET pair that are tethered together by either neutral (crowding) or two oppositely charged α-helices (ionic strength) in the linker region ( Liu et al, 2017b ). These environmental sensors have been investigated using ensemble averaging techniques such as time-resolved fluorescence ( Currie et al, 2017 ; Schwarz et al, 2019 ; Miller et al, 2020 ) and time-resolved anisotropy ( Currie et al, 2017 ; Leopold et al, 2019 ; Aplin et al, 2021 ) measurements. However, time-resolved fluorescence methods require expensive and specialized equipment as well as sophisticated users for experimental design and data analysis.…”

Section: Introductionmentioning

confidence: 99%

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Molecular Brightness Approach for FRET Analysis of Donor-Linker-Acceptor Constructs at the Single Molecule Level: A Concept

Kay

Aplin

Simonet

et al. 2021

Front. Mol. Biosci.

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In this report, we have developed a simple approach using single-detector fluorescence autocorrelation spectroscopy (FCS) to investigate the Förster resonance energy transfer (FRET) of genetically encoded, freely diffusing crTC2.1 (mTurquoise2.1–linker–mCitrine) at the single molecule level. We hypothesize that the molecular brightness of the freely diffusing donor (mTurquoise2.1) in the presence of the acceptor (mCitrine) is lower than that of the donor alone due to FRET. To test this hypothesis, the fluorescence fluctuation signal and number of molecules of freely diffusing construct were measured using FCS to calculate the molecular brightness of the donor, excited at 405 nm and detected at 475/50 nm, in the presence and absence of the acceptor. Our results indicate that the molecular brightness of cleaved crTC2.1 in a buffer is larger than that of the intact counterpart under 405-nm excitation. The energy transfer efficiency at the single molecule level is larger and more spread in values as compared with the ensemble-averaging time-resolved fluorescence measurements. In contrast, the molecular brightness of the intact crTC2.1, under 488 nm excitation of the acceptor (531/40 nm detection), is the same or slightly larger than that of the cleaved counterpart. These FCS-FRET measurements on freely diffusing donor-acceptor pairs are independent of the precise time constants associated with autocorrelation curves due to the presence of potential photophysical processes. Ultimately, when used in living cells, the proposed approach would only require a low expression level of these genetically encoded constructs, helping to limit potential interference with the cell machinery.

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Crowding Effects on Energy-Transfer Efficiencies of Hetero-FRET Probes As Measured Using Time-Resolved Fluorescence Anisotropy

Cited by 21 publications

References 76 publications

FRET Analysis of Ionic Strength Sensors in the Hofmeister Series of Salt Solutions Using Fluorescence Lifetime Measurements

FRET Analysis of Ionic Strength Sensors in the Hofmeister Series of Salt Solutions Using Fluorescence Lifetime Measurements

Quantification of FRET-induced angular displacement by monitoring sensitized acceptor anisotropy using a dim fluorescent donor

Molecular Brightness Approach for FRET Analysis of Donor-Linker-Acceptor Constructs at the Single Molecule Level: A Concept

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