Abstract
Förster resonance energy transfer (FRET) is a powerful tool for the visualization of molecular signaling events such as protein activities and interactions in cells. In its different implementations, FRET microscopy has been mainly used for monitoring single events. Recently, there has been a trend of extending FRET imaging towards the simultaneous detection of multiple events and interactions. The concomitant increase in experimental complexity requires a deeper understanding of the biophysical background of FRET. The presence of multiple acceptors for one donor affects the well-known formalism for FRET between two molecules, increasing distance sensitivity through mechanisms that have become known as the ‘antenna’ and ‘surplus’ effect. We will discuss the nature of these effects and present the imaging methods that have been used to unravel the combined transfer rates in the multi-protein interactions of multiplexed FRET experiments. Multiplexing strategies are becoming invaluable analytical tools for the elucidation of biological complexes and for the visualization of decision points in cellular signaling networks in physiological and pathological conditions.
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Introduction
When in immediate molecular proximity, the energy levels of fluorescent molecules can couple by Förster resonance energy transfer (FRET). This coupling can be measured in a microscope and provides a sensitive and robust metric for the interaction of the biomolecules carrying the fluorescent labels. The benefits for the life sciences lie in the fact that protein signaling and effector networks operate, in large parts, through conformational changes and the binding and unbinding of protein components. FRET allows the direct visualization of these decisive events through a variety of microscopy methods.
The cellular signaling network consists of multiple interconnecting and simultaneously occurring single events that, in the end, lead to a unified cellular response. FRET is used to entangle its working, but most FRET studies restrict themselves to the visualization of one signaling event by a FRET biosensor labeled with one FRET fluorophore pair. However, the correlation of several individual events over different cells is complicated by the inhomogeneity in cellular responses. For this reason, the last ten years has seen a rise in popularity in the extension of FRET measurements to the simultaneous detection of several events with multiple fluorophores and biosensors in a single cell. This ‘multiplexed’ detection has involved the parallel read-out of multiple single biosensors for interactions and signaling events, as well as structural studies on the composition of large multi-protein complexes and the detection of multiple conformations of molecules.
Typical FRET biosensors for the detection of single events are genetically encoded intramolecular sensors consisting of a single molecule, often a protein domain labeled with one donor and one acceptor fluorophore, that responds on a conformational change or cleavage. Intermolecular FRET designs are based on two interacting proteins, each labeled with either donor or acceptor fluorophores, for the detection of protein complex formation or their modifications. Both types of sensor also form the basis for the experimental designs of FRET multiplexing (Fig. 1).
Parallelization approaches have been reported in which simultaneously ongoing signaling reactions are followed by the expression of several intramolecular FRET sensors in one cell (Fig. 1a). Such a multiplexing experiment was performed by Piljic and Schultz (2008). They managed to simultaneously monitor three calcium-dependent signaling events by the combination of a cytosolic sensor for calcium/calmodulin-dependent protein kinase IIα, a membrane-bound sensor for protein kinase C, and a translocating FRET sensor based on annexin A4. Similarly, several ratiometric intramolecular sensors for the simultaneous monitoring of changes in the intracellular levels of various second messengers (Niino et al. 2009, 2010) and protein kinase A (PKA) activity (Aye-Han et al. 2012; Woehler 2013) were detected in parallel.
Further studies show the detection of combinations of enzymes and other small cellular analytes in the same cell, e.g., Src and MT1-MMP activities (Ouyang et al. 2010); caspase-3 activity and Ca2+ dynamics (Ding et al. 2011); and caspase-3 activity together with pH and redox co-factors (Sergeeva et al. 2017). In all these studies, the read-out of the individual sensors is based on the spectral separation of compatible and orthogonal FRET pairs.
To overcome spectral contamination, a multi-read-out approach using the additional dimension of fluorescence lifetimes in combination with spectral separation was used to discriminate Ras activity from a spectral ratiometric chameleon Ca2+ sensor (Grant et al. 2008). Another multiparameter study detected fluorescent lifetime changes of TN-L15, a genetic FRET calcium sensor, alongside homo-FRET detection by anisotropy of an AKT domain as an indicator of 3′-phosphoinositide accumulation (Warren et al. 2015). Recently, both the spectral and lifetime characteristics of a newly developed FRET donor, the monomeric cyan-excitable red fluorescent protein (mCyRFP1), were exploited to simultaneously monitor two signaling events (Laviv et al. 2016).
Irrespective of the popularity of the parallel approach of intramolecular sensors, other experimental designs for the detection of multiple conformational and intermolecular protein interactions are under active development. An extension of the multiplexing designs for intramolecular reporters involves consecutive ‘three-fluorophore’ or ‘two-step’ FRET (Maliwal et al. 2012; Watrob et al. 2003) (Fig. 1b). This approach has been used to address multiple conformational states within a molecule. In this case, one single molecule contains three fluorophores that form two consecutive FRET pairs. Furthermore, switching FRET was used to probe multiple distances in protein–DNA complexes (Uphoff et al. 2010). These studies mostly involve single-molecule FRET detection (smFRET) in order to circumvent the inhomogeneity of the reaction that complicates the interpretation in ensemble measurements.
Intermolecular ensemble measurements for multiple FRET detection by ‘three-fluorophore’ FRET using separate labeled proteins have predominantly involved the visualization of up to three interactions in a protein complex. Here, up to three individual protein components are each labeled with one fluorophore, which undergo combined energy transfer between them, such as the combination cyan, yellow, and red fluorescent proteins (Fig. 1c).
The first investigation of this kind in living cells was by Galperin et al. (2004), who showed the ternary interaction of proteins in Rab5-EEA.1 microdomains of endosomes and the interaction of EGFR with the adaptor protein Grb2 and the tyrosine phosphoprotein Cbl. A similar approach was then used to investigate the dimerization of the transcription factor C/EBPα and its interaction with the heterochromatin protein 1α (HP1α) (Sun et al. 2010).
Other ‘three-way’ or ‘triple-color’ FRET investigations were used to resolve binary interactions for the following set of protein triples: the adapter proteins SLP-76, Nck, and the guaninine nucleotide exchange factor Vav1 (Pauker et al. 2012); the actin-regulating complex consisting of WIP and WASp with the kinase PKCθ (Fried et al. 2014); and a small actin-regulating network involving N-WASP, actin, IQGAP1, and the small Rac1 and Cdc42 G-proteins (Wallrabe et al. 2015). Using spectral unmixing and deconvolution, the multiple protein interactions of HIV viral-like particles were imaged in three dimensions using fusion constructs of the HIV-Gag protein (Scott and Hoppe 2016).
Another major application of multi-fluorophore FRET is the determination of the stoichiometries of protein complexes. The biologically relevant metric in these cases is the quantity of complexes of a defined composition in a cell. Using spectral unmixing, FRET coupling in mixed donor–acceptor complexes was resolved (Raicu 2007; Singh et al. 2013; Stoneman et al. 2016).
The challenges of multiplexing FRET approaches lie, on the one hand, in expanding the number of different fluorophores that can be combined and, on the other hand, on the interpretation of the FRET data. Perhaps the popularity of the parallel use of single-molecule reporters in a multiplexing design, despite the technical challenges of increased spectral contamination, lies in the relatively easy accessibility of the FRET responses and their interpretation, as each sensor can be addressed individually. A more complicated situation presents itself for the detection of several protein conformations or several interactions in protein complexes, as the individual FRET responses likely influence each other. Nevertheless, these sensing schemes can provide unique event coincidence and stoichiometric information. The increasing complexity in the FRET detection and analysis that accompanies the development of such sophisticated multiplexing designs requires a deeper insight into the biophysics of the FRET phenomena and its detection methods.
Background: FRET between two molecules
FRET is the non-radiative transfer of excited state energy by dipole coupling between fluorophores that are in extreme close vicinity. For molecules with matching energies, resonance between the electron shells of a donating and accepting molecule causes the transfer of excited state energy. As a consequence, the donating molecule returns to the energetic ground state and the accepting molecule is raised to the excited state without being excited directly.
The nature of the coupling process is extremely dependent on distance, limiting FRET to short distances of up to maximally 10 nm for most biologically relevant fluorophores. This is the same order of magnitude as the length scale of proteins. Its extreme distance dependence and short range make FRET an ideal tool for probing protein–protein interactions, modifications, and conformational changes.
It was Förster’s seminal contribution to realize that the probability for two molecules to possess matching vibrational energy levels depends on the product of their frequency spectra, i.e., the degree of overlap between the donor emission spectrum and the acceptor absorption spectrum (Förster 1946, 1948). He introduced a transition probability function called the ‘overlap integral’, which describes the density of states of the excited donor and the acceptor that may be coupled and undergo isoenergetic energy transfer.
The overlap integral was the missing puzzle piece on the route to the FRET equation (Förster 1951) that is used today to predict and quantitatively describe FRET coupling with high precision. This equation (Eq. 1) describes the rate of energy transfer k T from the excited donor to the acceptor, as can be obtained from experimentally accessible variables:
in which κ 2 is a geometrical factor describing the relative orientation between the donor and acceptor transition dipoles, Q D is the donor quantum yield in the absence of FRET, n is the refractive index of the medium, N A is Avogadro’s number, r is the fluorophore separation distance, τ D is the donor lifetime in the absence of FRET, f D (λ) is the fluorescence spectrum, normalized to unity, and ϵ A (λ) is the acceptor absorption spectrum normalized to its molar extinction coefficient.
We will not expand on the derivation or historical background of this famous equation, for which we refer to van der Meer (2013) and Wouters (2013). However, it is important to discuss some of its components and their relation to the energy transfer rate, as these have direct consequences for FRET coupling between two molecules and for the expansion of FRET theory to include multiple acceptors per donor, as is the case for many implementations of multiplexed FRET.
Energy transfer rate, FRET efficiency, and lifetime
The energy transfer rate k T (in units s−1) describes the probability of the donor de-excitation (‘decay’) by losing energy through FRET. The other decay paths are through emission of a photon, as given by the radiative rate Γ, and through non-radiative energy losses by interactions with the environment, as given by the non-radiative rate k nr .
The fraction of all decay transitions to occur through FRET is given by the FRET efficiency E (ranging from 0 to 1, or 100%). This is equal to the ratio of the transfer rate over all rates combined (Eq. 2). The inverse of the sum of all rates is the (average) time it takes the excited state to return to the ground state. This is called the lifetime τ.
The lifetime of the excited state of the donor (τ D,no FRET ) is the inverse of the sum of the radiative, non-radiative, and—when present—energy transfer rate (τ D,FRET ) (Eq. 3):
The donor lifetime scales with the FRET efficiency. When the transfer rate increases, the FRET efficiency increases, and the time the donor spends in the excited state decreases. Lifetime measurements, therefore, provide direct insight into the de-excitation rates that act on the donor.
Interfluorophore distance and orientation
The Förster equation (Eq. 1) shows that FRET possesses a sixth-order dependence on separation distance. The typical distance range for FRET between a donor and acceptor is 1–10 nm. The distance dependence of FRET in a given fluorophore pair can be expressed in a critical also called Förster distance R 0. This is the distance r = R 0 at which the transfer rate equals the radiative plus non-radiative rate, and where the FRET efficiency is 0.5 (50%). From the Förster equation, this distance equals:
so that the transfer rate and FRET efficiency can be expressed in terms of distances:
These equations (Eq. 5) show why FRET is often called a ‘molecular ruler’, as the FRET rate and efficiency depend very sensitively on distance on a molecular length scale.
Realistic experimental values for FRET efficiencies in the life sciences typically lie between ∼50 and 5%, i.e., \( {R}_0\le r\le 1\frac{1}{2}{R}_0 \) (Fig. 2). As R 0 for common FRET pairs lies around 5 nm, a 5% change in FRET efficiency, which can be detected with confidence in FRET microscopy, corresponds to distance changes in the range of Angstroms.
A word of caution, however, is in order when distances are calculated from FRET efficiencies. The reason is that R 0 depends on the relative dipole orientation κ 2 (Fig. 2). The exact value(s) of κ 2 between interacting fluorophores in an experiment is not known a priori, but its limits can be estimated from the depolarization of fluorescence (Dale et al. 1979). With this information, accurate distance measurements can be obtained. Its value depends on the angles between the donor and acceptor dipoles and ranges from 0, for a perpendicular orientation, to 4 for a collinear orientation.
A value of \( {\kappa}^2=\frac{2}{3} \) is typically used for the calculation of R 0 of a FRET pair, as this corresponds to the statistical average of all possible orientations. Strictly speaking, this assumption only holds when the fluorophores are entirely rotationally free. However, a value for \( {\kappa}^2 = \frac{2}{3} \) is also acceptable in a regime in which the orientation of at least one of the fluorophores is fully random or mobile and leads to a small error in most cases (van der Meer 2002). At high degrees of immobility, however, distance estimations can suffer from large errors.
An instructive example of the influence of κ 2 on the FRET efficiency is the CFP-YFP fusion construct Cy11.5, in which the last 11 amino acids of CFP and the first five of YFP were removed. This head-to-tail construct has an expected interchromophore distance equal to the long axis of the fluorescent protein barrel, i.e., ∼4 nm, but sports a FRET efficiency of 98% (Shimozono et al. 2006). This high FRET efficiency cannot be explained from distances and the underlying cause should, rather, be sought in a preferred orientation of the fluorophores with κ 2 close to 4 (see also Fig. 2).
Therefore, especially for large fluorescent proteins (∼27 kDa) that are genetically fused to a protein of interest, caution should be exercised. Nevertheless, the distance dependence is on a scale that fully permits the binary detection of protein interactions and conformational changes. Considering its extreme distance sensitivity on the sub-nanometer scale, FRET microscopy can be counted as one of the optical super-resolution microscopy techniques.
FRET with multiple acceptors: going beyond one-on-one
The Förster equation (Eq. 1) holds true for the transfer of energy from one donor to one acceptor. In FRET experiments that use multiple fluorophores, it no longer accurately describes the distance dependence and magnitude of FRET, with consequences for its quantification.
Antenna effect: increase in distance sensitivity
When more than one acceptor is within reach of a donor, the probability for FRET coupling increases with the number of acceptors. For n identical equidistant acceptors with a single donor, R 60 effectively multiplies by n, leading to a change of (1/n)r 6 in the distance term. As a consequence, the distance sensitivity of FRET increases with the presence of multiple acceptors per donor without a real change in molecular distance (Fábián et al. 2010; Maliwal et al. 2012; Walczewska-Szewc et al. 2013 (Figs. 3 and 4a).
This distance-dependent increase is called the ‘antenna’ effect, as it increases the ‘sensitivity of reception’ of the donor energy. Clearly, for non-identical acceptors, the effect depends on the distances and R 0 values of the individual participating acceptors. Furthermore, one should keep in mind that the antenna effect is not limited to multiplexing experiments, but can also occur in intermolecular single-sensor FRET cases in which antibodies or probes that are labeled with multiple organic dyes are used, or where oligomers are formed.
A special limiting case of the antenna effect is for a donor approaching an (infinite) planar distribution of acceptors, e.g., for biomembranes. The distance dependence now assumes a fourth power relationship with the distance of approach and depends on the density of acceptors ρ in the membrane. In this case, the distance term becomes (2/πρ)r 4, with ρ in the number of acceptors per square nanometer when R 0 is in nanometers (Bastiaens et al. 1990; Kuhn 1972; Wouters 2013) (Fig. 3).
The increased distance sensitivity due to multiple acceptors becomes particularly apparent at distances between 1 and 1.5 times R 0, i.e., the typical distance range in FRET microscopy measurements. Especially for the planar condition, the main utility of FRET, its extreme distance dependence on the molecular scale, is threatened as it adds significant sensitivity in this lower FRET efficiency range. In membranes, acceptor expression levels can be reached that severely distort the familiar highly stringent distance relationship.
The antenna effect is reflected in the resulting transfer rate that equals the sum of the individual transfer rates, the so-called ‘kinetic model’ of FRET with multiple acceptors. It also increases the FRET efficiency.
At this point, it is already noteworthy to mention that the kinetic model illustrates the difference between FRET efficiencies and transfer rates (Eq. 6) as an experimental measure for energy transfer with multiple acceptors. Transfer rates from individual D → A 1 and D → A 2 measurements add to produce the transfer rate in the constellation A 1 ← D → A 2. In contrast, the measured, apparent, FRET efficiencies for the single pairs do not add and the sum will not be equal to the measured FRET efficiency of both acceptors. For biological applications in which the donor might couple with a single or both partners, or switch between these modes, transfer rates are, therefore, useful parameters, as they are additive and linear with acceptor coupling.
FRET surplus
In addition to the antenna effect, another phenomenon appears to increase the FRET efficiency even further. When using constructs containing multiple Venus acceptors for a single Cerulean donor, Koushik et al. (2009) observed that the FRET transfer rate in this construct exceeded the sum of the rates with the individual acceptors. This effect was named ‘FRET surplus’.
The cause of the enigmatic surplus FRET is not obvious and was discussed in terms of unknown FRET pathways. It can be explained from the statistical nature of the distribution of κ 2 values of the two competing FRET reactions (Fig. 4b). Assuming a random static or fully dynamic regime, and identical and equidistant acceptors, the sum of both rates would represent an equal chance for each acceptor to engage in FRET upon every donor excitation event. The overall average κ 2 for each FRET reaction D → A 1 and D → A 2 is 2/3. However, the κ 2 values for both D–A pairs will very likely not be the same in time at every donor excitation cycle and the pair with higher κ 2 value will have a higher chance of coupling. Due to this selection bias, the overall average κ 2 of a complex will be higher than the value of 2/3 for the D:A = 1:1 condition, increasing the combined FRET rate in the multi-acceptor complex. It is to be expected that this biased ‘sampling’ influence is greatest for the increase from 1 to 2 acceptors and then diminishes. Furthermore, the effect is expected to be largest for equal FRET rates of the individual couples.
To illustrate the effect of a selection bias of the orientation factor on FRET, we performed a simple simulation (Fig. 5). It is based on the assumption that the probability of selecting a κ 2 value from multiple identical and equidistant acceptors is proportional to their magnitudes at each excitation cycle (see legend of Fig. 5). This implies a selection bias towards the acceptor with the higher κ 2 value and, with this, an increase of k T exceeding the sum of the individual transfer rates. By increasing the numbers of acceptors, the model shows a first initial steep increase in the average κ 2, which approaches ∼1.35, corresponding to a doubling of the cumulative FRET rate (≈ 2(k T1 + k T2)). A donor with two equally FRET-competent acceptors already exhibits a ∼40% increase in FRET. This is in excellent agreement with the published data for a D:A = 1:2 construct (Koushik et al. 2009).
Detection and quantitative analysis of multiplexing FRET
The strength of FRET coupling is usually quantified as a FRET efficiency. The FRET efficiency, typically expressed as a percentage, is a useful and intuitive measure, as it corresponds to the fractional reduction in donor fluorescence intensity, in donor lifetime, and in the number of molecules that undergo FRET. The different FRET microscopy techniques of acceptor photobleaching, fluorescence lifetime imaging microscopy (FLIM), and sensitized emission, the latter optionally combined with spectral unmixing, provide this information and have all been used for the detection of FRET efficiencies in multiplexing experiments.
Nevertheless, in cases where multiple acceptors modify FRET coupling, it might be advantageous to work with the transfer rates, as these are additive. The measured FRET efficiencies as defined in Eq. 6 are not linear and, moreover, even ‘level off’ at higher values due to the inclusion of the transfer rate in the denominator. Consequently, efficiencies are less sensitive than energy rates over a large range of FRET coupling strengths and do not add for the purpose of FRET quantification of the multiplex condition. In the paper that first described the FRET surplus effect (Koushik et al. 2009), FRET efficiencies were transformed to transfer rates to show that the multi-acceptor constructs exhibited a transfer rate that exceeded the sum of the control duplex constructs.
A particularly useful parameter for FRET quantification that we would like to introduce is the ‘normalized transfer rate’ k ′ T obtained by normalization of the transfer rate to the sum of the radiative and non-radiative rates:
In contrast to transfer rates, the normalized transfer rate can be easily experimentally determined, similar to the FRET efficiency, by acceptor photobleaching microscopy and by FLIM:
in which ΔF D denotes donor dequenching upon acceptor photobleaching, F D is the donor fluorescence after photobleaching, and F DA is the quenched donor fluorescence in the presence of the acceptor, i.e., before acceptor photobleaching. Similarly, Δτ D is the difference between the donor lifetime without (τ D ) and with FRET to an acceptor (τ DA ).
Most importantly, the normalized transfer rate has the same additive and linear properties as the transfer rate for FRET with multiple acceptors. Furthermore, it exhibits a direct relation between distance and the R 0 distance (Eq. 7), in which a value of 1 denotes a separation distance equal to R 0. A related normalized transfer rate k T /Γ has been proposed as a measure for FRET previously (Jares-Erijman and Jovin 2003; Roberti et al. 2011). They adopted this metric for the latter reason. However, we wish to maintain the distance relationship to the classical Förster distances, whereas k T /Γ requires the definition of a modified R 0 .
If required, the FRET efficiencies and the normalized transfer rates can be interconverted, for example to calculate the cumulative FRET efficiencies in a multiplexing experiment. The relationship between the FRET efficiency and the normalized transfer rate is given by:
Especially, the surplus effect presents a difficulty for FRET quantification. Together with the antenna effect, it, however, presents an elegant diagnostic tool for the unequivocal determination of complex (or oligomer) formation. When a donor-labeled component interacts with two different acceptor-labeled components A1 and A2, and the biological question relates to the DA1A2 complex formation with possible DA1 and DA2 intermediates, the antenna and surplus effects exclusively operate on the ternary complex DA1A2. When FRET exceeds the sum of DA1 and DA2 measurements, ternary complex formation is a fact. Both the antenna and surplus effects can be clearly detected in the donor channel as donor yield and lifetime changes and can, therefore, be effectively read out by donor-only methods as acceptor photobleaching and FLIM (Fig. 6).
In contrast, in multiplexing experiments based on sensitized emission measurements, the energy transfer is detected from changes in acceptor fluorescence. Usually, binary interactions between the individual donor acceptor pathways (DA1 and DA2) are sampled in such experiments. However, the emission detected for each of the acceptor channels is effectively reduced, as the energy transferred from the shared donor to the additional acceptor does not contribute to the measured sensitized emission (Eq. 10). In analogy to Eq. 6, the FRET efficiencies in sensitized emission are:
Consequently, the FRET efficiency measured by sensitized emission of acceptor 1 (E se, A1 ) is lowered due to the ‘antenna’ effect by the presence of acceptor 2, indicated by the suffix A2 (E A2 se,A1 ). The same holds true for sensitized emission measured from acceptor 2. For the same reason, the surplus effect will result in a further reduction of the FRET efficiency, leading to its underestimation.
The FRET quantification of sensitized emission measurements using different acceptors has been solved and used for the study of multi-protein interactions. We refer to several excellent papers on this topic: Fried et al. (2014), Pauker et al. (2012), Scott and Hoppe (2016), Sun et al. (2010), and Wallrabe et al. (2015). Sensitized emission FRET with multiple identical acceptors, e.g., in oligomerization experiments, on the other hand, behaves similar to donor FRET measurements.
In conclusion, both the donor-only and the sensitized emission approaches provide relevant information and both have underlying antenna and surplus effects. However, in sensitized emission FRET, the surplus effect is not experimentally accessible, as a measurement of sensitized emission on the combined non-identical acceptors is typically not performed. This situation is different in the donor FRET methods, where the transfer of energy to all acceptors combined is measured.
Conclusion
Sophisticated Förster resonance energy transfer (FRET) multiplexing schemes are increasingly being used to elucidate multiple protein interactions in single cells. These assays hold the promise to solve the dynamic connectome of strategic sets of proteins, for instance to understand decision points in signaling events, as well as the stoichiometry of multimeric protein complexes. However, their quantitation is complicated by the fact that FRET between a single donor and multiple acceptors behaves differently from the known one-on-one condition. In addition to a predictable ‘antenna’ effect that is based on the summation of the transfer rates that act on the donor, quantification is confounded by a ‘surplus’ effect, likely caused by the statistical selection of a more favorable relative dipole orientation among the acceptors. These effects have an influence on the quantification of FRET independent of the microscopy method used. At the same time, they can be taken as powerful diagnostic indicators for true FRET multiplexing of donor molecules. As acceptor-based FRET measurements predominantly provide information on the coupling strength to a specific spectrally distinct acceptor, and donor FRET measurements, especially FLIM, provide easy access to rates that permit the evaluation of the surplus effect, we expect to see an increase in multimodal, spectrally resolved, and quantitative FRET microscopy approaches in the future that incorporate the strengths of the individual methods.
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This work was supported by the DFG Research Center “Nanoscale Microscopy and Molecular Physiology of the Brain”. Both authors GB and FSW declare that they have no conflict of interest.
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Gertrude Bunt declares that she has no conflict of interest. Fred S. Wouters declares that he has no conflict of interest.
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Bunt, G., Wouters, F.S. FRET from single to multiplexed signaling events. Biophys Rev 9, 119–129 (2017). https://doi.org/10.1007/s12551-017-0252-z
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DOI: https://doi.org/10.1007/s12551-017-0252-z