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    • 专利摘要:
    The present invention relates to a method for detecting a reversibly photocommutable fluorescent species (P) at a high frequency, and more specifically to a method for detecting at least one reversibly photocomputable fluorescent species, comprising a step of illuminating a sample containing a species fluorescent light reversibly photocompatible with a first illumination light (FEX1), wavelength and periodically modulated to a pulsation ω and with a second illumination light (FEX2) of wavelength λ2 different from λ1, periodically modulated to the pulsation ω, the second illumination light being modulated in antiphase with respect to said first illumination light.
    公开号:FR3055704A1
    申请号:FR1658163
    申请日:2016-09-02
    公开日:2018-03-09
    发明作者:Jerome Querard;Thomas Le Saux;Ludovic Jullien
    申请人:Centre National de la Recherche Scientifique CNRS;Universite Pierre et Marie Curie Paris 6;Ecole Normale Superieure;
    IPC主号:
    专利说明:

    Holder (s): NATIONAL CENTER FOR SCIENTIFIC RESEARCH, PARIS 6 PIERRE AND MARIE CURIE UNIVERSITY Public establishment, SUPERIOR NORMAL SCHOOL Public establishment.
    Extension request (s)
    Agent (s): MARKS & CLERK FRANCE General partnership.
    FR 3 055 704 - A1 (34) METHOD FOR THE DETECTION OF REVERSIBLY PHOTOCOMMUTABLE FLUORESCENT SPECIES AT HIGH FREQUENCY.
    The present invention relates to a method for detecting a reversible photocommutable fluorescent species (P) at high frequency, and more precisely a method for detecting at least one reversible photocommutable fluorescent species, comprising a step consisting in illuminating a sample containing a reversibly photocommutable fluorescent species with a first lighting light (FEX1), of wavelength and periodically modulated at a pulse puls and with a second lighting light (FEX2) of wavelength λ 2 different from λ υ modulated periodically at pulsation ω, the second lighting light being modulated in antiphase with respect to said first lighting light.
    METHOD FOR DETECTION OF REVERSIBLY PHOTOCOMMUTABLE FLUORESCENT SPECIES AT HIGH FREQUENCY
    The invention relates to a method for detecting reversible fluorescent photocommutable high frequency species. Such a process has numerous applications, in particular in chemistry, in biology and in the field of environmental measurements and screening.
    "Species" means a chemical species such as a molecule or complex, or a physical object such as a nanoparticle. The term “reversibly photocommutable species” (“photoswitchable” or “photoconvertible” in the English literature) means a species having at least two distinct states, having different fluorescence properties, and being able to pass from one state to another. reversibly by the effect of light. Examples of reversibly photocommittable fluorescent species are the protein "Dronpa" and the complex "Spinach - DFHBI" ("Spinach" being an RNA aptamer and DFHBI a fluorogenic probe). These species can, in particular, be used as probes or markers. Other examples of reversibly switchable fluorescent species can be azo derivatives or protein scaffolds.
    Imaging, and more specifically fluorescence microscopy, has become an indispensable tool in biology, but also in other disciplines such as materials science. Its applications, however, are limited by the ability to observe a signal of interest in a background of fluorescence or noise. This problem is particularly acute in in vivo, animal or plant imaging applications, in which the fluorescent markers to be detected are dispersed in a complex autofluorescent and / or diffusing medium; the useful signal is then drowned in an intense background noise.
    Another limitation of fluorescence detection and imaging techniques lies in the width of the spectral band of the fluorophores generally used in relation to the width of the visible spectral band: it is difficult to selectively detect more than four fluorescent markers in the same sample, because their emission spectra tend to overlap.
    To overcome these limits, patent application WO 2015075209 A1 discloses a method using reversible photocommutable fluorescent probes, in which a sample is illuminated, containing a species of photocommutable fluorophore with periodically modulated light. The component of the intensity emitted by the fluorophores at the same pulse is then detected, in phase quadrature with respect to the excitation wave. This method makes it possible to selectively detect certain reversibly photocommutable fluorophores by minimizing, under certain conditions calculated analytically as a function of the characteristics of the fluorophore, the noise produced in traditional methods by autofluorescence and / or diffusion of the medium of the sample. One of the problems with this method is the frequency with which successive images are acquired. The different reversibly photocommutable fluorescent species used in the state of the art pass from an activated state to their initial state not activated in a thermally induced manner: the characteristic time of this transition is for example 5 to 10 seconds and corresponds to the time to acquire an image using this method. This time scale is too large to carry out a large number of measurements relevant in biology.
    Another technique of the prior art is disclosed in the article by YenCheng Chen et al. (Chen, YC, Jablonski, AE, Issaeva, I., Bourassa, D., Hsiang, JC, Fahrni, CJ, & Dickson, RM, 2015, Optically Modulated Photoswitchable Fluorescent Proteins Yield Improved Biological Imaging Sensitivity, Journal of the American Chemical Society, 137 (40), 12764-12767) which proposes a fluorophore detection method implementing a heterodyne excitation of a fluorescent species reversibly photocommutable by two sources of monochrome laser illumination of different excitation wavelengths. This technique offers an empirical choice of the parameters for measuring the fluorescence of one species, which does not allow this type of measurement to be easily transposed to other species. In addition, the signal-to-noise ratio when measuring a reversibly photocommutable fluorescent species is not optimal. Finally, the disclosed method does not instruct those skilled in the art how to observe two reversibly photocommutable fluorescent species at the same time.
    The invention aims to remedy the aforementioned drawbacks of the prior art, and more particularly to:
    • image a sample by discriminating several different fluorophores;
    • allow fluorophores to be imaged using a technique to eliminate high-frequency scattering / auto-fluorescence noise;
    • in general, selectively and quantitatively image one or more fluorescent probes in a mixture.
    An object of the invention making it possible to achieve this goal, partially or totally, is a method for detecting at least one reversible photocommutable fluorescent species, comprising the following steps:
    (a) illuminating a sample containing said or at least one said reversibly photocommutable fluorescent species with a first illumination light, of wavelength λ 1; and modulated periodically at a pulse ω and with a second lighting light of wavelength λ 2 different from λ 1; periodically modulated at said pulsation ω;
    (b) detecting fluorescence radiation (FLU) emitted by said sample thus illuminated; and (c) extracting the amplitude of the intensity component of said fluorescence radiation having the same periodicity as said first lighting light modulated periodically and in phase quadrature with respect to it;
    • said second lighting light being modulated in antiphase with respect to said first lighting light and • the average intensity of said first lighting light, the average intensity of said second lighting light, and their pulsation ω being chosen so as to approach a maximum of said amplitude of the intensity component of said fluorescence radiation. For example, the amplitude can take a value equal to at least 75%, preferably 80%, more preferably 90% of the maximum.
    According to a particular embodiment of such a method, at least one said reversibly photocommutable fluorescent species can have a first and a second chemical state, at least one of said states being fluorescent, said or each said reversibly photocommutable fluorescent species being capable of being converted from said first state to said second state by a first photo-induced reaction, then returning to said first state by a second photo-induced reaction, and said first lighting light can have an average intensity Z ° and be modulated at a pulse ω and said second lighting light have an average intensity of 7 ° with:
    (<712.1 + <721, l) Il = (<7l2.2 + <721.2) 1% and ω = 2 © 12.1 + σ 2 ι, ι) 1 ° where σ ΐ2, ιΛ ° and ^ 21.1 ^ 1 are, respectively, the kinetic constants of said first and said second photo-induced reaction by said first lighting light; and where σ 122 Ι 2 and σ 212 Ι 2 are, respectively, the kinetic constants of said first and said second photo-induced reaction by said second lighting light.
    Furthermore, the average intensity of said first lighting light, the average intensity of said second lighting light, and their pulsation ω can also be chosen so as to ensure a minimum contrast between said amplitude of the component of intensity of said fluorescence radiation and the amplitude of a fluorescence intensity component, having the same periodicity, from an interfering species.
    Another object of the invention is a method for detecting at least two reversibly photocommutable fluorescent species having different dynamic properties, comprising the following steps:
    (a) illuminating a sample containing each said reversibly photocommutable fluorescent species with a first light of wavelength lighting and modulated periodically according to a first function summing at least two first lighting components modulated by pulses ω ,, each said pulsation ω, of each said first lighting component being associated with a said reversibly photocommutable fluorescent species, and being different from the other said pulse or pulses ω,; and lighting with a second lighting light, of wavelength λ 2 different from λ 1; and periodically modulated according to a second function summing at least two second lighting components modulated by said pulsations ω ,, each said pulsation ω, of each said second lighting component being equal to a said pulsation ω, of a said first component lighting;
    (b) detecting fluorescence radiation (FLU) emitted by said sample thus illuminated;
    (c) extracting each amplitude (algebraic) of the intensity component of said fluorescence radiation exhibiting the same pulsation ω, as each said lighting component, and in phase quadrature with respect to each said first lighting component;
    • for each said pulsation ω ,, each said second lighting component modulated by said pulsation ω, being in antiphase with respect to each said first lighting component modulated by said pulsation ω,;
    • and the average intensity of said first lighting light, the average intensity of said second lighting light, and said pulsations being chosen so as to approach a maximum of each said amplitude of the component of intensity of said fluorescence radiation.
    According to particular embodiments of such a process:
    Each said reversibly photocommutable fluorescent species can have a first and a second chemical state, at least one of said states being fluorescent, each said reversibly photocommutable fluorescent species being capable of being converted from said first state to said second state by a first photo-induced reaction, then to return to said first state by a second photo-induced reaction, and said first lighting light can have an average intensity of 7 ° and be periodically modulated according to a said first function, and said second lighting light can have an average intensity Z 2 ° with P ° ur each said reversibly photocommutable fluorescent species:
    © 12,1 + ^ 21, l) Il = © 12,2 + ^ 21,2) ^ 2 where σ ΐ2, ι ^ ι θΐ σ 2ΐ, ι ^ ι are, respectively, the kinetic constants of said first and of said second photo-induced reaction by said first lighting light of said species; and where σ 122 Ι 2 and σ 212 Ι 2 are, respectively, the kinetic constants of said first and said second photo-induced reaction by said second lighting light of said species.
    For each so-called pulsation corresponding to a so-called reversibly photocommutable fluorescent species, it is possible to have:
    Mi = 2 (^ 12.1 + σ 2 ι, ι) ΐ
    where σ 12 , ι / ι ° and σ 21Λ / ° are, respectively, the kinetic constants of said first and said second photo-induced reaction by said first lighting light of said species. Advantageously, the ratio between at least two said pulsations ations, can be strictly greater than 10.
    During said step a), said sample can be illuminated by at least one substantially monochromatic lighting light.
    Said steps b) and c) can be implemented by synchronous detection of said fluorescence radiation.
    The method can also include the following step: d) determining the concentration of said or at least one said reversibly photocommutable fluorescent species from the intensity component of said fluorescence radiation extracted during said step c).
    Said or at least one said reversibly photocommutable fluorescent species can be chosen from: a photochromic fluorescent protein; and a complex of a biomolecule with a fluorogenic probe.
    The sample may contain biological material.
    Yet another object of the invention is a fluorescence imaging method (and in particular fluorescence microscopy) implementing such a detection method. In this case, said sample can comprise a living organism, and at least one element chosen from the presence and the concentration of a said reversibly photocommutable fluorescent species can be measured from the intensity component of said fluorescence radiation extracted during of said step c) without taking a sample from said living organism.
    Said lighting light can comprise part of daylight and said part of daylight can participate in the light intensity received by said reversibly photocommutable fluorescent species by remaining less than or equal to the average intensities of said lighting lights .
    The invention will be better understood and other advantages, details and characteristics thereof will appear during the explanatory description which follows, given by way of example with reference to the appended drawings in which:
    FIG. 1 illustrates a method for detecting a reversible photocommutable fluorescent species P according to the invention;
    FIG. 2 illustrates a diagram presenting a theoretical calculation of the response of a reversibly photocommutable fluorescent species P in the case of an embodiment belonging to the prior art;
    FIG. 3 illustrates a diagram presenting a theoretical calculation of the response of a reversibly photocommutable fluorescent species in an embodiment of the invention;
    FIG. 4 illustrates an embodiment of the invention making it possible to image several fluorescent species reversibly photocommutable during the same image detection;
    FIG. 5 illustrates a digital simulation corresponding to the quantification of a reversible photocommutable fluorescent species in the presence of X interfering compounds;
    Figure 6 is a graph illustrating photochemical properties of a set of reversibly photocommutable fluorescent species;
    Figure 7 is a set of photographs illustrating an experimental comparison between achievements of the prior art and an embodiment of the invention;
    FIG. 8 illustrates a detection of the fluorescence image of a cell according to an embodiment of the invention;
    FIG. 9 illustrates a system implementing a method according to an embodiment of the invention.
    FIG. 1 illustrates a method for detecting a reversible photocommutable fluorescent species P according to the invention. The method comprises lighting a sample E with a first lighting light FEX1, of wavelength and a second lighting light FEX2, of wavelength λ 2 , different from λ ± . Each of the lighting lights FEX1, FEX2 is preferably substantially monochromatic, that is to say that its spectrum has a single maximum intensity, and / or a spectral width less than or equal to 50 nm.
    The reversibly photocommutable fluorescent species P has two different states exchangeable under the action of light. It can be a photochromic fluorescent species, or any other system whose dynamic behavior can be reduced to an exchange between two states under the action of light; these states can correspond to different stereochemical configurations of a molecule, to a linked / unbound state of a complex, etc. In FIG. 1, the first state - thermodynamically more stable - is indicated by 1 and represented by a solid square; the second state - thermodynamically less stable - is indicated by 2 and represented by a hollow square. These two states have different brightnesses. For the sake of simplicity, and by way of nonlimiting example, it can be considered that only state 1 is significantly fluorescent.
    The sample E, and more precisely the species P which it contains, illuminated by a first lighting light FEX1 and by a second lighting light FEX2, emits fluorescence radiation FLU whose intensity is itself also, modulated and can be broken down into:
    a component in phase with the first lighting light FEX1, indicated in the figure by l F in ; and a quadrature component with the excitation beam, indicated in the figure by l F 0Ut . Patent application WO 2015075209 A1 discloses the interest and the basis for observing the component l F 0Ut when observing species P.
    The dynamic behavior of a reversibly photocommutable fluorescent species P can be described as follows. Under the illumination of a species P by a light of intensity / (/) comprising two components ZiCt) and / 2 (Ό "corresponding respectively to a first light of illumination FEX1, of wavelength and to a second lighting light FEX2, of wavelength λ 2 , the dynamic behavior of the species P can be described by the following two-state exchange:
    / -12 (/) - 2 / -21 (/) in which state 1, thermodynamically more stable, is converted by a photochemical reaction into a thermodynamically less stable state 2 with a kinetic constant ^ 12 (/) = ^ 124 / 1 (/) - 0 / 2.2 / 2 (/), e t can return to the more stable initial state 1 by a photochemical and / or thermal process with a kinetic constant ^ 21 (/) = 0-214 / 1 (/) + ^ 21.2 / 2 (/) + ^ 21, in which σ ΐ2.ιΑ (/), σ ΐ2.2 ^ 2 (/), <T2i, i7i (i), ^ 21.2 ^ 2 ^ ) represent the photochemical contributions and ^ 21 the thermal contribution to the speed constants, σ ΐ2, ι being the photoconversion cross section from state 1 to state 2 illuminated by light FEX1, σΐ2 - 2 being the cross section of photoconversion from state 1 to state 2 illuminated by light FEX2, σ 2ΐ4 being the cross section of photoconversion from state 2 to state 1 illuminated by light FEX1 and σ 2ΐ, 2 being the cross section from photoconversion of state 2 v ers state 1 lit by the FEX2 light. All of these constants define the behavior of species P.
    By assumption, the system is uniformly lit or can be considered homogeneous at all times. The evolution of concentrations 1 (state 1 concentration of species P) and 2 (state 2 concentration of species P) can then be described by the following system of equations:
    and dt dt “fei2 (£) 1 + fei (X) 2
    M.2 C © 1 fei® '2 (2) (3)
    Considering that the sample E is suddenly lit by two sources of constant lighting, of wavelength and λ 2 respectively , the lighting is characterized by the intensity 7 (ί) = I® + 1% = 1 ° e t kinetic constants can be written as:
    & 12 NOT - _ 1.0 _ k 0, lP - ^ 12 - ^ 12.1 + Λχ2.2 7 J (4) = 1.0 _ pO i; 0 | λ, Δ^ 21 - ^ 21.1 + ^ 21.2 + ^ 21- (5)K '12, l tO - σ 12, Ul J (6) ^ 21.1 70 - σ 21.1-ίι J (7) ^ 12.2 rO- ^ 12.2 ^ 2J (8) ^ 21.2 rO- <721.2 ^ 2. (9)
    Considering that the initial state contains only species 1, the concentrations of 1 and 2 change according to:
    1θ - 1
    -2 exp i —q12 · (10)
    WHERE ^ 12 + ^ 21 (11) corresponds to the relaxation time of a reversibly photocommutable fluorophore and 1 ° and 2 ° at concentrations 1 and 2 in the photostationary state reached at time τ ° 2 We also have:
    1 '
    Early, (12) or:
    ^ 12
    LO / ΰ 2 χ (13) and the total concentration of species P is P tot = 1 + 2.
    It is possible to analyze the response in fluorescent emission, or FLU fluorescence radiation of a reversibly photocommutable fluorescent species P when it is subjected to two periodically modulated lighting lights FEX1, FEX2, corresponding to embodiments of the invention.
    In general, it can be considered that a reversibly photocommutable fluorescent species P is subjected to an illumination comprising two components: a periodic illumination ^ (t) at the wavelength and an illumination / 2 (0 at the wavelength λ 2 , which can be constant in a different embodiment of the invention, or periodically modulated in all of the embodiments of the invention. In the most general case, we can write:
    J (i) = I ± (t) + h (t) (35) and
    Ij (t) - Ij [1 + ahj (t)] (36) and with j = 1 or 2. In equation (36), a corresponds to the amplitude of the light modulation and / i 7 (t) corresponds to periodic functions. Equations (4) and (5) become here:
    ki2 (t) = fc 2jl [1 + ahi (i)] + / c 2; 2 [1 + "M ^)] (37) - ^ li.i [1 + ahi (t)] + fc 21 , 2 [1 + cià 2 (/)] + k ^ i
    L (38)
    By introducing a function / (t), we can develop the expression of the 10 concentrations as follows:
    = 2 ° + af (t) = 1 ° - af (é) (39) (40) and
    The system of differential equations governing the temporal evolutions of the 15 concentrations 1 and 2 can be solved with equations (2) and (3) to obtain:
    df (x dx where:
    = - / (a ) + K - b 2 / (x)] hi (x) + [a 2 - b 2 / (x)] h ^ x} (41) '-
    20 -> 1 T 12 n ,, ο Λθ 0 α ι ^ 12 ^ 12.1 ^ .2 bx = za (cr 121 + σ 2 ΐ, ΐ) / θ τ θ 2 (42)(43)(44) „J1 λΟ Ω a 2 - P12 ^ 12,2'12 (45) b 2 = α (σχ 2 , 2 + Cr 2 l, 2) - ^ 2 T 12 (46) 25 and or : .i) _ L.0 lO _ 7.0 QÜ P12 - ^ 12 1 - r 21 z (47)
    (48)

    (49) respectively designate the speed of the reaction corresponding to equation (1) in the steady state (with 1 ° and 2 ° given in equation (12)) and the differences in the relative contributions of the means of the modulated lights (respectively Z ° and 7 °) to the kinetic constants leading respectively from state 1 to state 2 or from state 2 to state 1.
    After the relaxation time τθ 2 , a steady state is established, in which / (%) is a continuous periodic function. More generally, / (%) can be a periodic function. In the various embodiments of the invention, the modulation of lighting FEX1, FEX2 can be carried out by a fundamental pulse ω or two fundamental pulses (ω-t and ω 2 ) or at least two fundamental pulses, each of the different fundamental pulses being called in this case by a generic term ag.
    In a first case, the Fourier series corresponding to / (%) can be written in the form:
    + OG fUx) = a ° + V cos ("M + siu (" M] / 2 = 1
    (50) where:
    (51) and where a n, cœ and b n, S111 denote the amplitudes of the n-th components of the Fourier series.
    In the second case, the Fourier series corresponding to / (%) can be written in the form:
    -jib. φοο / <e , e 2 æ) = a ° + 2 J] siu [(, / ^ i »/ A 2 ) .r]} n = —og m = —go (52) where:
    = (53)
    Θ2 = ω 2 τ ^ (54) and where a °, a n ' m ' cos and b n ' m ' sin correspond to the amplitudes of the 0-th and {n, m} th components of the Fourier series. a ° and / or a n ' m ' cos and / or b n ' m ' SLn can be extracted from equation (41) by identifying the components of the same order.
    The set of equations obtained can be transformed so as to explain the concentration modulations for all the pulses. We can then write:
    +00 = 2 ° + "[ 2 n, sm sin (ηθχ) + 2 n, COS cos n = l (55) +00 = i ° - a [ 2 n, sin sin (ηθχ) + 2 n, cos cos (η $ τ)] n = l (56)
    OR
    2.o, sin
    2 n, C ° S
    2 ° + ο; οθ, (57) 1 ° - aa ° (58) j-tqsin _ ^ n.sin (59) , n.cos ~ n.cos —1 - - a · (60)
    or :
    +00 +00 = 2 ° + a τι —— 00 m —— oo (61) + 0Q +00 = ι ° - α ^ 2 η '™ ! ® “8Ϊη [(ηθι + roéh) æ] + 2 n ' m ' cos eos [(n0i + ra ^) æ] J n —— OG 1TI— - QQ (62) where
    2 ° = 2 ° + aa °} i ° = 1 ° - aa °J n, m, stn _ _ ^ n, m, sin _ yn, m, sin n, m, c05 _ _ ^ n, m, cos _ „N, m, cos Cl '·
    (63) (64) (65) (66)
    You can also express the fluorescent intensity. We define, in equation (67), the observable Oj corresponding to the observation at wavelength with j = 1 or 2:
    Oj (i) = Qyjl (t) + Q2, j2 (t ') zgyx either, by extracting the fluorescence emission (£) in equation (68):
    / F (f) = Οι (ί) / χ (ί) + O 2 (i) ^ W · (68)
    We have, with the time dependence given by equations (55) and (56):
    OC
    Oj (t) = [ü ” , sm sin {ηθχ) + D” ' COb cos {ηθχ).
    n = l L (69) with and
    Qijl ° + ¢ 2 ../ 2 ° + (<5 2j - Q /, /) yy ° (70) ^ n.sm (Q 2 .j - Qu) a6 ' sin(71) , ^ n, cos (Qij - Qi J (72) oonx = 3® + E [: ï | , sm sin {ηθχ) + 0 | ' co & cos {ηθχ)
    n = l (73)
    While the expressions for the amplitudes of the terms 0 7 (t) are generic, the expressions for the amplitudes of the terms / F (t) vary with the time dependencies of the lighting.
    We have, with the time dependencies of 1 (t) and 2 (t) given by equations (61) and (62):
    4-00 4-00 □, · (/} = £ / + | o ' m ' slll sin [(;; (/! +) .R] - eus ./·] J n = —ôo m = —oc with:
    (74) - “L Q'2,7'2 ( '+ (Q'2.7 - Qï.j} ΠΟθ (75) = (Q 2j . _ Qli -) (76) D „, m .cos = ÇQ 2 J - Ql j ) (77)
    and
    4-oo 4-00
    Jg - y ^ y ^ | ) G m ' i, ln sill [(»4i L- /////oi./·] J- 3g m ' roi, COS.
    n —— oc m = ”© G (78) in which, in the same way, the expressions of the amplitudes of the terms 0 7 (t) are generic, the expressions of the amplitudes of the terms / F (t) vary with the time dependencies lighting.
    The inventors first considered cases in which the modulations of the two lighting amplitudes are low, and noted ε in place of a thereafter. This case makes it possible to linearize the equations and to derive analytical expressions.
    In embodiments belonging to the prior art, sinusoidal modulations of one of the two lights are produced, for example the lighting FEX1 at the wavelength oscillating around an average intensity 7 ° at the pulsation ω and with a small amplitude εΙ ° (ε "1) on which a constant intensity illumination 7 ° is superimposed on a wavelength λ 2 . We then have:
    = if [1 + £ sin (ωί)] + if / ii (t) = sin (wi) (80 )
    WO = 0- (81)
    By developing at first order the expression of the light disturbance, equation (41) becomes:
    = -f (θχ) + (82)
    After the relaxation time τ ° 2 given in equation (11), we can derive:
    and:
    = i ° = 1 - (u 7-} î,) - „0 Λ ü
    - A ° “ Δ Ι2,1 '(83) (84) ^ Ptot (ΐ ^ Λ-yl-Çh) (85) (1 -i-Ji fy 1 + ζ (ωτ | 2) (86) Λ 0 21 12 ωτ 12 c “12.1 ,, —v-Uot = (Qu 1 ° + Q 2 , i2 °) / + (Qi, 2 1 ° + Q 2. 2 2 °) 4 .1“ “= î {( Who 0 + Qj, j2 °) / ° + [(Q ,,, - Q 24 ) 1 ° + (Q,, - Q2.2) 4] 1 ““ '} (88) 2 (87) ~ | i .eos
    O = 7 [(Ql.l - Q'2.1) Il + (Ql.2 - Q2.2) h] ^ l.COS (89)
    By using two different wavelengths, the exchanges between states 1 and 2 are essentially governed by photochemical contributions by choosing the average intensities (/ f, / 2 0 ) so that : Gsid / f + g 2L2 7 § »k £ L
    FIG. 2 illustrates a diagram presenting a theoretical calculation of the response of a reversibly photocommutable fluorescent species P in the case of an embodiment belonging to the prior art. The diagram in FIG. 2 illustrates the value of the normalized amplitude of the quadrature oscillations of
    I JL Vj'Jo
    J-norm e n as a function of the control parameters Ζθ / ζΡ and ω / Zf. This case corresponds to lighting FEX1 at the wavelength oscillating around an average intensity Z ° at pulsation ω and with a small amplitude εΙ ° (ε "1) to which a constant lighting of intensity Z2 is superimposed on a wavelength λ2. The reversibly photocommutable fluorescent species P considered is “Dronpa-2”, the kinetic parameters of which the inventors have measured, corresponding to σ12, ι = 196 m 2 .mol ' 1 , σ2ι, ι = 0 m 2 .mol' 1 , σ12; 2 = 0 m 2 .mol ' 1 , σ21; 2 = 413 m 2 .mol' 1 and k 21 = n-2 -1 - = 100 —- ¾1,4.10 s and with 1 σι 2 , ι + σ - · 2ΐ, ι.
    In this case, Hnorml presents a singular maximum when the following two resonance conditions are met:
    (90) (91)
    This optimization results from an independent optimization of the terms
    Δ / = ε / Ρ di and + ^ 2 ] of equation (86). I ° is the change Δ2 0 d u steady state 2 after a jump amplitude Δ / ι = εΙ ι. It is maximized when the kinetic constants of the photochemical reactions induced by the two lights are equal. The second optimized term, ^ / P + ^ 2 ], is maximized by adjusting the pulsation ω to the relaxation time τ 2 so as to have 0 = 1. When ω »1 / ti 2j replacement is slow compared to the variations in lighting and the couple {1,2} does not have enough time to respond, so as to make disappear the terms î 1, sin and i 1, cos . Conversely, when ω < 1 / ' Γ ί 1 2, i 1 ^ 08 is canceled, and concentrations 1 and 2 oscillate in phase with the modulation of the lighting. More generally and in all of the embodiments of the invention, the average intensity of said first lighting light (FEX1), the average intensity of said second lighting light (FEX2), and their pulsation ω are chosen so as to maximize the amplitude of the intensity component of said fluorescence radiation (FLU) in phase quadrature with respect to the first illumination light.
    In embodiments of the invention, the two lighting lights FEX1, FEX2 are modulated sinusoidally (or more generally periodically), at the same pulsation puls. The inventors have discovered the possibility of increasing the first order amplitude of the response to lighting modulations of a species P compared to the case in which the second lighting light excites a species P with a constant intensity. We consider, by way of example, that / (t) comprises a superposition of two sinusoidal modulations of small amplitudes: on the one hand, at the wavelength around the mean intensity / f and at the pulsation ω and on the other hand, at the wavelength λ 2 around the average intensity 7 ° and at the pulsation ω. We consider :
    1 (1) = [1 + [1 +
    J hi (t) = sïii (üjî)
    J h2 ^ t) = sin (ωί + φ) with ε "1.
    (92) (93) (94)
    By developing the disturbance of lighting at the first order, / (^) = / 1 (^) + / 2 (^) is a solution of equation (41) when / i ($ Æ ) and are solutions of the following equation (95):
    tkv / (&) + ajfty (fe) (95) with respectively j = 1 or 2. We can notice that this equation is similar to equation (82). After the relaxation time τ ° 2 given in equation (11), we can derive:
    (96) (97) .i.sm, i, sra
    Οχ : d 2 (ces φ + Θ sin φ) j ....... j, ...... 02ι · + fi 2 , l.COS, l.COS dj.fi d 2 (sinφ - Θ cos φ)
    T ~ fi
    1 + fi 2 (98) (99) and 99 become:
    2 ^ 1, sin ^ i, sin ^ i.œs cos
    For species P used in embodiments of the invention, without limitation, the transition induced by photochemical effect from state 1 to state 2 (respectively from state 2 to state 1) is governed exclusively by wavelength lighting (respectively  2 ). Considering that the reaction kinetic constant from state 2 to state 1 is mainly governed by photochemistry, we can deduce that + = ”^ 2. The equations —- 1 —v [fl - cos φ) - Θ sin +1 i + e 2Lk ψ> (ioo)
    --h— W (1 - cos ω) + sin ipl + fi 2 v (101)
    2αχ
    1 + fi 2 (102)
    2a-, fi
    Equations (100) and (101) show that φ = π is typically favorable for increasing the amplitudes of the fluorescence response. Equations (100) and (101) then become:
    i.sin _ i.sin
    x. '- 1'' l.COS, l.COS _ + fi 2 (103) and the terms of the fluorescence intensities are:
    3 ° s = (Qi, il ° + Q 2 .i2 °) / + (<2l 2 1 ° + Q ^ '2 0 ) I) (104)
    3j sil * = ε {[(<3i.il 0 + Q2, i2 °) I 0 , - (Qi, 21 0 + Q 2 , 2 2 °) $}} + ε {[(Qu - Q2.1) I + (Qi, 2 - Q222) F i 1 '™} (1θ5)
    c “= ε [(Who - Qz.i) / + (Qi, 2 - ¢ 2.2) f2] i 1, c <> s · (106)
    In particular, the inventors have discovered that the lighting variation corresponding to equation (92) with φ = π qualitatively produces the same "1.COS results for J s with respect to a light excitation governed by equation (79 ) but with an amplitude which, in theory, is twice as great. This increase in amplitude makes it possible to solve several technical problems posed by the prior art, by selectively imaging a species P, obeying the resonance conditions given by equations (90) and (91), with greater resolution time and a higher signal-to-noise ratio. More generally, in all of the embodiments of the invention in which a first lighting light FEX1 is periodically modulated at a pulse ω and a second lighting light FEX2 is periodically modulated at the same pulse ω, the second FEX2 lighting light is modulated in antiphase, that is to say at φ = π with respect to the first FEX1 lighting light.
    FIG. 3 illustrates a diagram presenting a theoretical calculation of the response of a reversibly photocommutable fluorescent species P in an embodiment of the invention. The diagram in FIG. 3 illustrates the value of the normalized amplitude of the quadrature phase oscillations for a
    I, i, cos i _ i 1.00 s / η concentration I 1 (l-Uwvmi - I-1 - / OoîI), based on control parameters
    I2 / I1 and ω // °. This case corresponds to lighting FEX1 at the wavelength oscillating around an average intensity 7 ° at the pulsation ω and with a small amplitude ε / ° (ε "1) to which a lighting FEX2 is superimposed at the length of wave λ 2 oscillating around an average intensity / 2 ° at the pulsation ω and with a small amplitude ε / 2 (ε "1). The other parameters are similar to the parameters used in the embodiment corresponding to FIG. 2. In this case,
    X, COS j | J-twtm | presents a singular maximum when the two resonance conditions, corresponding to equation (90) and (91), are met, as in the embodiment illustrated in FIG. 2, but whose norm is substantially twice as large, resulting in a 4-fold increase in signal-to-noise ratio. The signal to noise ratio can be considered as a signal to interference ratio (SIR).
    FIG. 4 illustrates an embodiment of the invention making it possible to image several fluorescent species reversibly photocommutable during the same image detection. In this embodiment of the invention, a first lighting light FEX1 of wavelength is periodically modulated according to a first function summing at least two first lighting components modulated by pulsations ω ,, the pulsations being different from each other other. In the nonlimiting example illustrated in FIG. 4, the first lighting light FEX1 is modulated by a function summing a component of pulsation ωι and a component of pulsation ω 2 . Each of the pulsations ω, is associated with, or corresponds to, a reversibly photocommutable fluorescent species of the imaged sample E. In the case illustrated in FIG. 4, the pulsation ωι corresponds to the species P represented by a full square and an empty square, and the pulsation ω 2 corresponds to the species P 'represented by a full hexagon and an empty hexagon. The species P ”represented by a circle does not correspond to any particular pulsation. The sample is also lit with a second lighting light FEX2 of wavelength λ 2 , periodically modulated according to a second function summing at least two first lighting components modulated by the same pulses ω ,, that is to say say in the nonlimiting case of FIG. 4, by the pulses ωι and ω 2 .
    Analytically, we can consider, without limitation, that the intensity Z (t) of the lighting is a superposition of two sinusoidal modulations of small amplitudes, with pulses auxι and ω 2 , oscillating around an average intensity 7 ° at the wavelength and around an average intensity I 2 at the wavelength λ 2 . In other embodiments of the invention, the modulations can be periodic, of different forms, and of larger amplitudes. We consider :
    J (i) = if [1 + £ hi (t)} + Ιθ [1 + ε ^ 2 (/)] (121) ài (i) = sin (ωχί) + / 3 sin (u / 2Î) ( 12 2) / i2 (/) = ~ sin (α / χί) - β sin (α / 2 /) (123) with ε "1. In this case, 1 l 1 + ^ iW] corresponds to a first function and I 2 [1 + e / i2 (/)]) corresponds to a second function.
    By developing lighting disturbances to the first order, / (x) = Ιι (θ 1 χ) ^ β / 22 χ) is a solution of equation (41) when / i (0iæ) and / 2 (^ 2 ^) are solutions of the following equation (124):
    = -fj (0jx) + (α χ - a 2 ) sin (^ - x) dx JJJ (124) with respectively j = 1 or 2. After the relaxation time τ ° 2 , we can derive:
    2 ° = 2 ° (125) i ° = 1 ° (126) ^ 1.0, sin , 1.0, sin ^ 2)““ 1 + 0 (127) ^ 1.0, COS _ 1.0, COS ““ ^ 2.)“1 + 0 (128) 20.1.8111 _ Ύ 0.1, sin η (θ · ι - 0-2) 1 + ¾ 2 , t (129) 20, i, cos _ _ 0.1, cos a ^ -2 ·) @ 2~ 1 + 0 (130)
    Equations (127) to (130) lead to:
    2 i, o, sin
    Pl2 T 12 ( Δ 12.1 ^ 12.2) + (ωιτ 2 ) 2 ^ 12 ( Δ 12.1 Δ 12.2) ρ (1 + Ο 2 ιφ <* (131) ^ Χ, Ο, ίΟΗ ^ 1- ^ 12 / ¾ 7 ¾ (^ 13.1 = ^ 12, g) _ _ Kg ^ 1 7 ¾ (^ 13.1 ~ ^ 12, g) ρ.
    i + H <r ^ ii + <r i + ( W1 <r (132) o, i, sin _ .-. / AV'il ( Δ 2.1 ' Δ Ί -. ΐ)
    1+ (^ 27¾) 2 β-, χ, οοβ _ 0 ^ 1 ^^ 127¾ (^ 12.1 ~~ ^ 12.2) + Μ / ^ 12 ( Δ ! 2.Ι Δ Ι2.ΰ) ρ
    Ίΐ 4 · Λ- © Γ 14 Η-4) 2 Ιϋ! (133) q 4¾ (^ 12.1 - ^ 12.2) „(l + <f ι + Μ) 2 “ (134) and the associated terms of oscillating fluorescence emissions are:
    = (<2l, ll ° + Q2, l2 °) / + (Qi, 2l ° + 02.22 °) il (135) = ε {(<2i, i 1 ° + <32, i2 °) 1 ° - (Qi, 2 1 ° + Q 2 , 2 2 °) 1 °} + ε {[(Qu - o 2 , i) Ii + (Oi, 2 - 02,2) / ] I 1Asin } (136) l ^ = ε [(Οι, ι “Ο24) 7 + (Oi, 2 ~ ¢ 2.2) 12] i 1 ' 0 ' 1105 (137)
    V '™ = εβ {(Qi, il ° + Q 2 , i2 °) / - (Qi, 2 1 ° + Q 2 , 2 2 °) / 2 °} + ε {[(Οι, ι - 0 2 , i) 1 + (Oi, 2 - O 2 , 2 ) ι 0 ' 1 ' ™} 3 , (138)
    3 ° / '™ = £ [(.Ql, l ~ Q2. 1 ) li + (Ql, 2-Q2,2dl} T · ^.
    In this embodiment of the invention, the fluorescence response of the sample E to the superposition of two antiphase modulations of low amplitudes at two different pulses ωι and a> 2 allows the embodiments of the invention corresponding to the figures to be used 1 and 3 to simultaneously and selectively detect two species P 'and P. Advantageously, the photocommutable species share identical resonance conditions in light intensity 7 ° and 7 °, corresponding to equation (90). Advantageously, each of the photocommutable species is associated with the pulses ωι and a> 2 as defined in equation (91), and corresponding to the resonant pulsations of each of the species P 'and P ”. In particular, the expressions of fluorescence derived in equations (136) and (137) are similar to equation (107), but with an amplitude twice greater in the particular case of this embodiment of the invention in which < * i = allowing a selective and simultaneous detection of two distinct P 'and P species.
    Advantageously, the periodic modulations applied to the intensities of the first lighting light FEX1 and of the second lighting light FEX2 are not weak compared to the average intensity of its lighting lights. They can for example be of the same order of magnitude. In the case of periodic modulations of large amplitudes of the intensities of the lighting lights FEX1, FEX2, that is to say in the case where a <1, the inventors have discovered that the conditions described above remain valid. These validations were carried out by numerically calculating the different orders of truncated Fourier series whose corresponding functions were linearized in the previous cases considering low amplitudes of intensity modulation.
    The arrows in FIG. 4 illustrate different images Im obtained after post-processing of the intensity signal lF 0Ut . These images Im can be obtained by demodulation of the acquired signal associated with the pulsation ω, corresponding to the reversibly photocommutable species of interest.
    FIG. 5 illustrates a numerical simulation corresponding to the quantification of a species P in the presence of interfering compounds X. In the absence of information on the various fluorescent species present in a sample, it is possible to optimize the response of the first order in quadrature phase fluorescence lF 0Ut by choosing a triplet (Ζ ^, Ζθ, ω) which verifies the resonance conditions given in equations (90) and (91), so as to selectively and quantitatively image a species P among interfering species X, defined by the set of parameters
    in this case, do not be photocommutable, this case corresponding to the parameters σ 12ΧΧ = σ 21 <ίΛ = 0 (for i = 1 or 2) and k 2ix = 0. Figure 5 illustrates the case of a mixture of fluorophoric species reversibly switchable P, of which only state 1 emits fluorescence, characterized by the same brightness Q 1; 7 ·. In this case, a protocol consisting in illuminating at constant intensities Z ° gives a signal Ζθ proportional to the sum of the contributions of the different fluorophores, such as:
    or :
    X
    titration (223)

    (224)
    When the signal Ζθ is used to titrate P species, the result of the titration overestimates the total concentration P to t due to the contributions of the interfering species. On the other hand, the first-order quadrature response of phase ^ 1, ÇOS to lighting can be expressed:
    > l.cos titration
    X (225) where (226) t-) 1, cos ^ titration = Pt early f -, 1, COS! -y ( (JX / ^ tot, v "/, 1 _ A hVfot
    Z-, 1, COS l -p ' lp / -Pot, and makes it possible to determine P to t when the triplet of parameters (/ °, / θ-ω) is adjusted under the resonance conditions for a species P. indeed, the term lp C0S is maximum while the terms © cos are negligible. The signal from species P is predominant compared to that of the other interfering species, and the result of titration P ^ tration is approximately equal to Ptot Panel A in Figure 5 illustrates a numerical simulation of the normalized amplitudes 1 ampl / 1 ° ( illustrated by gray disks) and normalized amplitudes of lx , C0S / lp C0S (illustrated by black squares) for four equimolar mixtures including the target species characterized by the quintuplet (σ 12.1, σ 2ΐ, ι, σ 12 , 2, σ 21.2, k2i A ) and sixteen other interfering species. In each sample marked n, these interfering species correspond to the sixteen quintuplets (σ ι2, ι, χ, σ 2 ι, ι, χ, σ i 2 , 2, x, σ 21.2, x, k 2 i A ), whose four photochemical parameters differ by n orders of magnitude from (σ ι 2 , ι, σ 21.1, σ 12.2, σ 21.2) Figure 6 illustrates photochemical properties of a set of reversibly fluorescent species photocommutables. For each of the species considered, the resonance conditions according to equations (90) and (91) have been measured and are illustrated by absolute iso-value curves of the normalized amplitude of the quadrature response of first-order fluorescence phase quadrature . Curve (a) corresponds to the species "Dronpa >>, curve (b) corresponds to the species" Dronpa-2 ", curve (c) corresponds to the species" Dronpa-3 >>, the curve (d) corresponds to the “RS-FastLime” species, the curve (e) corresponds to the “Padron” species, the curve (f) corresponds to the “Kohinoor” species, the curve (g) corresponds to the species "rsEFGP" and the curve (h) corresponds to the species "rsEFGP2 >>.
    In one of the embodiments of the invention, the sample E is illuminated with two lighting lights of different wavelengths, and each of the lighting lights is periodically modulated, in order to image several reversibly selectively photocommutable species, such as illustrated in FIG. 4, the triplet / -Ρ, / θ, ω, being chosen for each of the species so as to maximize the component lF 0Ut of the fluorescence radiation.
    In a particular embodiment of the invention, one places oneself under the conditions of resonances imposed by the two average intensities of the lighting lights, that is to say according to the relation (σΐ2, ι + σ 2 ι, ι) / ι = (^ 12.2 + ^ 21.2) / 3 Graphically, this solution consists in imaging two reversibly photocommutable species whose resonance conditions can be illustrated by points substantially close to the same vertical line in FIG. 6.
    A variant of the invention consists in placing oneself under these conditions and in choosing two frequencies and ω 2 (in the case of a detection of two species P 'and P) verifying the conditions of resonances of each of the species. In other words, each pulse ω satisfies the condition ω = © 12.1 + <+21.1) Λ-This realization makes it possible to maximize the amplitude of each first order response in quadrature of phase in fluorescence lF 0Ut .
    Another variant of the invention consists in placing oneself under the conditions verifying the relation ( 0 ¾ 1 + σ 2ΐ, ι) / = (+12.2 + <+21.2) / °> t to choose two pulses of modulation of the lighting lights, each associated with a reversibly photocommutable species, whose ratio is, for example, strictly greater than 10, preferentially to 100. Indeed, when the relation (90) is verified, the ratio of the resonant pulsations proper to two species P ′ and P can be low, for example less than 10. In this case, by placing oneself in conditions verifying the relation (91), the amplitude lF 0Ut corresponding to each species is maximized, but the contribution of the interferences of an amplitude associated with one species on the other prevents obtaining an optimal contrast of a species vis-à-vis -vis the other. In this variant, it is possible to use the relation (106) to choose pulses for modulating the lighting lights FEX1, FEX2 so as to impose a ratio between the pulses greater than a predefined value, for example 10, to increase the contrast. .
    More generally, it is possible to deviate from the maximum amplitude of the fluorescence signal in order to increase the contrast with respect to one or more interfering species. One can for example maximize the amplitude of the fluorescence under constraint to ensure a minimum contrast, maximize the contrast subject to ensuring a minimum amplitude (generally expressed as a percentage of the maximum amplitude), or even determine a region of the parameter space (ω / h, h / b) ensuring both a sufficiently large amplitude and a sufficiently high contrast. Similarly, in the case where the aim is the detection of a single fluorescent species, it may be advantageous to deviate from the resonance conditions to improve the contrast with the fluorescence of interfering species, at the cost of a reduction. signal amplitude. Most often, however, we will choose lighting conditions ensuring a signal amplitude equal to at least 75%, preferably 80% and more preferably 90% of the maximum achievable.
    FIG. 7 is a set of photographs illustrating an experimental comparison between embodiments of the prior art and an embodiment of the invention.
    Panel A in FIG. 7 is a photograph illustrating cellular nuclei, marked by a species P. The photograph is produced, according to a method of the prior art, by imaging the signal l F 0Ut with a first light of illumination of wavelength = 480 nm periodically modulated, and with a second illumination light of wavelength λ 2 = 405 nm, of constant intensity.
    Panel B of FIG. 7 is a photograph illustrating the same cellular nuclei, marked by the same species P. The photograph is produced, according to a method of the prior art, by imaging the signal l F 0Ut with a first light of illumination of wavelength = 480 nm of constant intensity, and with a second illumination light of wavelength λ 2 = 405 nm modulated periodically.
    The panel C in FIG. 7 is a photograph illustrating the same cellular nuclei, marked by the same species P. The photograph is taken, according to a method embodiment of the invention, by imaging the signal lF 0Ut with a first light of illumination wavelength = 480 nm modulated periodically, and with a second lighting light of wavelength λ 2 = 405 nm modulated at the same period and in antiphase.
    In panel A in Figure 7, the intensities are doubled. In panel B of Figure 7, the intensities are multiplied by -2. The intensity peaks are substantially equal in all of the panels in the figure, illustrating the increase in signal, described in FIG. 3, during an embodiment employing two lights, periodically modulated in antiphase compared to modulated lighting periodically, or with periodically modulated lighting and a second lighting with constant lighting. The amplitude lF 0Ut measured, in embodiments of the prior art and / or in embodiments of the invention is algebraic: we can discriminate lF 0Ut measured by their absolute values and / or by their signs.
    FIG. 8 illustrates a detection of the fluorescence image of a cell according to an embodiment of the invention. In this example, the nucleus of the cell is marked by a species P, in this case "Dronpa-2". The mitochondria of the cell are marked by another P '"Padron" species. The species P '"Padron" is characterized by a dark state 1 and a fluorescent state 2. In this example, two modulation pulses are set. A ratio of 100 is imposed between the two modulation pulses. A first pulse, ηι 00 ω (£) -2) is associated with the species P '"Dronpa-2 >>; this pulse is greater than the resonance pulse of "Dronpa-2". A second pulse, ω (Ραάτοη), is associated with the species P "Padron"; this pulse is less than the "Padron" resonance pulse. The legends "Padron >>and" D-2 "on the left of the images indicate respectively a demodulation of the pulsed fluorescence signal associated with" Padron >> and "Dronpa-2 >>. The legends "P >>and" N >> to the right of the images indicate respectively that the amplitude represented by lF 0Ut is of positive sign (P) or negative (N).
    The left column of FIG. 8 illustrates images obtained according to an embodiment of the invention, by lighting with two lighting lights of different wavelengths modulated in antiphase, at the pulsation η 100 ω (£) - 2) . The nucleus of the cell is observed significantly, corresponding to a positive amplitude of lF 0Ut and to a demodulation at the pulsation corresponding to D-2.
    The middle column of FIG. 8 illustrates images obtained according to an embodiment of the invention, by lighting with two lighting lights FEX1, FEX2 of different wavelengths modulated in antiphase, at pulsation (eÇPadrori). The mitochondria of the cell are observed significantly, corresponding to a negative amplitude of lF 0Ut and to a demodulation at the pulse corresponding to Padron.
    The right column of FIG. 8 illustrates images obtained according to an embodiment of the invention, by lighting two lighting lights FEX1, FEX2 of different wavelengths, and modulated by components with pulses η οω (£) -2) and a> (Padrori), each component of the second lighting light FEX2 being in antiphase of the corresponding component of the first lighting light FEX1. We observe significantly both the nucleus of the cell, corresponding to a positive amplitude of lF 0Ut and a demodulation at the pulse corresponding to D-2 and the mitochondria of the cell, corresponding to a negative amplitude of lF 0Ut and to a demodulation at the pulse corresponding to Padron.
    FIG. 9 illustrates a system implementing a method according to an embodiment of the invention. This system, illustrated by way of nonlimiting example, comprises two light sources SLM1 and SLM2 each consisting of a light-emitting diode. The SLM1 light source is powered by an AM1 power source and the SLM2 light source is powered by an AM2 power source. The modulation of each of the light sources SLM1 and SLM2 is obtained by modulation of the respective power supply power by means of a GF function generator having two independent outputs. The emission of the light-emitting diodes being with broad band, the beams FEX1 and FEX2, emitted by SLM1 and SLM2 respectively, are collimated by lenses, then filtered by two optical filters before being directed on a sample, constituted by a microfluidic device DMF; for the sake of simplicity, the optical filters are not shown in the figure. The illuminated sample is observed, by its rear face, by an OBJ objective which collects the fluorescent radiation and focuses it in a FLU beam. The latter is filtered (filter F2) and directed, by an M mirror and an LF lens, onto the sensor of a CAM camera. A computer includes a processor PR controlling the camera CAM so as to detect in phase quadrature as described above. Advantageously, the acquisition frequency of the camera is commensurable with the modulation frequency of the sources FEX1, FEX2. To carry out simple detection and / or titration, without imaging, the CAM camera can be replaced by a point light sensor.
    权利要求:
    Claims (15)
    [1" id="c-fr-0001]
    1. Method for detecting at least one reversibly photocommutable fluorescent species (P), comprising the following steps:
    (a) illuminating a sample containing said or at least one said reversibly photocommutable fluorescent species with a first lighting light (FEX1), of wavelength A 1 ( and periodically modulated at a pulsation ω and with a second light of lighting (FEX2) of wavelength A z different from À 1 , periodically modulated at said pulsation ω;
    (b) detecting fluorescence radiation (FLU) emitted by said sample thus illuminated; and (c) extracting the amplitude (l F 0Ut ) of the intensity component of said fluorescence radiation (FLU) having the same periodicity as said first lighting light (FEX1) modulated periodically and in phase quadrature with respect to to her ;
    • said second lighting light (FEX2) being modulated in antiphase with respect to said first lighting light (FEX1) and • the average intensity of said first lighting light (FEX1), the average intensity of said second lighting light (FEX2), and their pulsation ω being chosen so as to approach a maximum of said amplitude of the intensity component of said fluorescence radiation (FLU).
    [2" id="c-fr-0002]
    2. Method according to the preceding claim wherein at least one said reversibly photocommutable fluorescent species (P) has a first and a second chemical state, at least one of said states being fluorescent, said or each said reversibly photocommutable fluorescent species (P) being susceptible to be converted from said first state to said second state by a first photo-induced reaction, then to return to said first state by a second photo-induced reaction, and in which said first lighting light has an average intensity 1% and is modulated at a pulse ω and said second lighting light has an average intensity / ° with:
    (<712.1 + <721.1) - ^ 1 = (<712.2 + <721.2) - ^ 2 and ω = 2 (σΐ2, ι + σ 2 ι, ι) where σ 12ι1 / ° and are, respectively, the kinetic constants of said first and said second photo-induced reaction by said first lighting light (FEX1); and where at 12 , 2 J 2 ^ 21.2 ^ 2 are, respectively, the kinetic constants of said first and said second photo-induced reaction by said second lighting light (FEX2),
    [3" id="c-fr-0003]
    3. Method according to one of the preceding claims, in which the average intensity of said first lighting light (FEX1), the average intensity of said second lighting light (FEX2), and their pulsation ω are also chosen to so as to ensure a minimum contrast between said amplitude of the intensity component of said fluorescence radiation (FLU) and the amplitude of a fluorescence intensity component, having the same periodicity, from an interfering species.
    [4" id="c-fr-0004]
    4. Method for detecting at least two reversibly photocommutable fluorescent species (P) having different dynamic properties, comprising the following steps:
    (a) illuminating a sample containing each said reversibly photocommutable fluorescent species (P) with a first light of illumination (FEX1) of wavelength and periodically modulated according to a first function summing at least two first lighting components modulated by pulses ω ;, each said pulse αη of each said first lighting component being associated with a said reversibly photocommutable fluorescent species (P), and being different from the other said other pulse (s) αη; and illuminate with a second lighting light (FEX2), of wavelength λ 2 different from Λ 1 ( and periodically modulated according to a second function summing at least two second lighting components modulated by said pulses οη, each said pulsation ω, of each said second lighting component being equal to a said pulsation ωι of a said first lighting component;
    (b) detecting fluorescence radiation (FLU) emitted by said sample thus illuminated;
    (c) extracting each amplitude (If 011 *) from fa component of the intensity of said fluorescence radiation having the same pulsation αη as each said lighting component, and in phase quadrature with respect to each said first lighting component ;
    • for each said pulsation ω · ,, each said second lighting component modulated by said pulsation ωι being in antiphase with respect to each said first lighting component modulated by said pulsation ωι;
    • and the average intensity of said first lighting light (FEX1), the average intensity of said second lighting light (FEX2), and said pulses being chosen so as to approach a maximum of each said amplitude of the intensity component of said fluorescence radiation.
    [5" id="c-fr-0005]
    5. Method according to the preceding claim wherein each said reversible photocommutable fluorescent species (P) has a first and a second chemical state, at least one of said states being fluorescent, each said reversible photocommutable fluorescent species (P) being capable of being converted. of said first state to said second state by a first photo-induced reaction, then to return to said first state by a second photo-induced reaction, and in which said first lighting light (FEX1) has an average intensity 7 ° and is modulated periodically according to a said first function, and said second lighting light (FEX2) has an average intensity / 2 ° with P ° ur each said reversibly photocommutable fluorescent species (P):
    (σΐ2, ι + σ2ΐ, ι) Ιθ = (0 + 2.2 + 021.2) Ιθ where σ ΐ2, ι / ι ° θΐ σ 2ΐ, ι / ι are, respectively, the kinetic constants of said first and of said second photo-induced reaction by said first lighting light (FEX1) of said species; and where σ 122 Ι $ and σ 212 Ι 2 are, respectively, the kinetic constants of said first and said second photoinduced reactions by said second lighting light (FEX2) of said species.
    [6" id="c-fr-0006]
    6. Method according to the preceding claim, in which, for each said pulsation ω, corresponding to a said reversibly photocommutable fluorescent species (P):
    Mi = 2 (û- 12 ,! + 0-2 ^) / 1 ° where σ 12 , ι / ι ° and σ 21Λ / ° are, respectively, the kinetic constants of said first and said second photo-induced reaction by said first lighting light (FEX1) of said species.
    [7" id="c-fr-0007]
    7. The method of claim 5 in which the ratio between at least two said pulsations ω, is strictly greater than 10.
    [8" id="c-fr-0008]
    8. Method according to one of the preceding claims wherein, during said step a), said sample is illuminated by at least one substantially monochromatic lighting light.
    [9" id="c-fr-0009]
    9. Method according to one of the preceding claims in which said steps b) and c) are implemented by synchronous detection of said fluorescence radiation.
    [10" id="c-fr-0010]
    10. Method according to one of the preceding claims also comprising the following step:
    d) determining the concentration of said or at least one said reversibly photocommutable fluorescent species (P) from the intensity component of said fluorescence radiation extracted during a said step c).
    [11" id="c-fr-0011]
    11. Method according to one of the preceding claims, in which said or at least one said reversibly photocommutable fluorescent species is chosen from:
    a photochromic fluorescent protein; and a complex of a biomolecule with a fluorogenic probe.
    [12" id="c-fr-0012]
    12. Method according to one of the preceding claims, the sample of which comprises biological material.
    [13" id="c-fr-0013]
    13. Method according to one of the preceding claims, in which said lighting light (FEX) comprises part of the daylight and in which said part of the daylight participates in the light intensity received by said fluorescent species. reversibly photocommutable (P) while remaining less than or equal to the average intensities of said lighting lights (FEX1, FEX2).
    [14" id="c-fr-0014]
    14. Fluorescence imaging method implementing a detection method according to one of the preceding claims.
    [15" id="c-fr-0015]
    15. Method according to the preceding claim in which said sample can comprise a living organism, and in which at least one element chosen from the presence and the concentration of a said reversibly photocommutable fluorescent species (P) is measured from the component of the intensity of said fluorescence radiation extracted during said step c) without taking a sample from said living organism.
    1/6
    2/6 lm
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    同族专利:
    公开号 | 公开日
    EP3506951A1|2019-07-10|
    WO2018041588A1|2018-03-08|
    US10718712B2|2020-07-21|
    US20190212268A1|2019-07-11|
    FR3055704B1|2018-10-05|
    JP2019532280A|2019-11-07|
    JP6858843B2|2021-04-14|
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    EP3839484A1|2019-12-17|2021-06-23|Centre National de la Recherche Scientifique|Method for detecting a reversibly photoswitchable label in a sample|
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    优先权:
    申请号 | 申请日 | 专利标题
    FR1658163|2016-09-02|
    FR1658163A|FR3055704B1|2016-09-02|2016-09-02|METHOD FOR DETECTING REVERSIBLY PHOTOCOMMUTABLE FLUORESCENT SPECIES AT HIGH FREQUENCY|FR1658163A| FR3055704B1|2016-09-02|2016-09-02|METHOD FOR DETECTING REVERSIBLY PHOTOCOMMUTABLE FLUORESCENT SPECIES AT HIGH FREQUENCY|
    JP2019512269A| JP6858843B2|2016-09-02|2017-08-10|A method for detecting fluorescent species that can be reversibly optical-switched at high frequencies|
    PCT/EP2017/070307| WO2018041588A1|2016-09-02|2017-08-10|Method for detecting fluorescent species that are reversibly photoswitchable at a high frequency|
    US16/330,040| US10718712B2|2016-09-02|2017-08-10|Method for detecting fluorescent species that are reversibly photoswitchable at a high frequency|
    EP17755452.4A| EP3506951A1|2016-09-02|2017-08-10|Method for detecting fluorescent species that are reversibly photoswitchable at a high frequency|
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