Mechanosensitive Fluorescent Probes to Image Membrane Tension in Mitochondria, Endoplasmic Reticulum, and Lysosomes

Goujon, Antoine; Colom, Adai; Straková, Karolína; Mercier, Vincent; Mahecic, Dora; Manley, Suliana; Sakai, Naomi; Roux, Aurélien; Matile, Stefan

doi:10.1021/jacs.8b13189

Cited by 177 publications

(251 citation statements)

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“…This implied that the effective fluorescence quantum yield of the planarized cascade switch 4 should be F So > 60 %, higher than the F So > 38 %oforiginal 1 (Table 1). According to FLIM images of L d and L o GUVs, [5,6] fluorescence lifetimes of cascade switch 4 were shorter than the original 1 (Figure 4c,F igure S17 in the Supporting Information, Table 1). However, like intensity ratios,l ifetime increases upon planarization from L d to L o membranes were slightly higher for 4 (t Lo /t Ld = 2.07) than for 1 (t Lo /t Ld = 1.90;T able 1).…”

Section: In Memory Of Koji Nakanishimentioning

confidence: 96%

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A Chalcogen‐Bonding Cascade Switch for Planarizable Push–Pull Probes

et al. 2019

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Planarizable push-pull probes have been introduced to demonstrate physical forces in biology.However,the donors and acceptors needed to polarizem echanically planarized probes are incompatible with their twisted resting state.T he objective of this study was to overcome this "flipper dilemma" with chalcogen-bonding cascade switches that turn on donors and acceptors only in response to mechanical planarization of the probe.T his concept is explored by molecular dynamics simulations as well as chemical double-mutant cycle analysis. Cascade switched flipper probes turn out to excel with chemical stability,red shifts adding up to high significance,and focused mechanosensitivity.M ost important, however,i st he introduction of an ew,g eneral and fundamental concept that operates with non-trivial supramolecular chemistry,solves an important practical problem and opens aw ide chemical space.Planarizable push-pull (PP) chromophores have been introduced [1] as mechanosensitive [2] fluorescent membrane probes [1][2][3] to image membrane tension [4] in living cells. [5,6] The current best is constructed around twisted dithienothiophene (DTT) dithienothiophene S,S-dioxide (DTTO2) conjugates ( Figure 1a,D ' = S, A' = SO 2 ). [7] Thet wo "flippers" [7] are twisted out of coplanarity by repulsion between the methyls (light blue circles) and the s holes (dark blue ovals) [8][9][10][11] on the sulfurs next to the connecting bond (Figure 1b,l eft, 1). The PP system is prepared first with "sulfide" donors and "sulfone" acceptors in the DTT and the DTTO2b ridges, respectively (Figure 1b, 8,9). Conjugation of DTT and DTTO2u pon mechanical co-planarization then turns on this intrinsic PP system and shifts the excitation maximum to the red (Figure 1b,r ight). Thee mission maximum is nearly mechanoinsensitive because the probes emit only from the planar form. [12] To achieve significant red shifts upon planarization in the ground state,a dditional PP donors Da nd acceptors Aa re required (Figure 1a). These exocyclics ubstituents represent atrue dilemma because in the twisted resting state,the DTT donors and DTTO2 acceptors,a tl east partially decoupled from each other and equipped with extra Da nd A, could become too rich and too poor in electron density,respectively, and decompose easily (Figure 1a). Because both DTTs and DTTO2are comparably electron-rich, [13] this problem is more pronounced on the DTT side.T herefore,Dand As hould ideally turn on only in response to flipper planarization. Sulfides,p reviously introduced as covalent PP turn-on donors, [12] failed to afford operational probes. [14] Non-covalent 1,4-chalcogen bonds (1,4-CBs) [8][9][10][11] as in 1 were more successful, also because spontaneous degradation into reactive Figure 1. a) Flipper dilemma and b) CB cascade switch:a)Inplanarizable PP probes, exocyclic donors D D and acceptors A A are needed in planar but incompatiblew ith twisted form. b) Twisting of the central bond (1)turns off PP D D (2,r ed circle), and A A (3,b lue circle) because Lewis base Y( 5)hardly ...

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Section: In Memory Of Koji Nakanishimentioning

confidence: 96%

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confidence: 99%

A Chalcogen‐Bonding Cascade Switch for Planarizable Push–Pull Probes

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“…[4][5][6][7] In particular,u nderstanding fast processes such as signal transduction requires the abilityt om easure reaction kinetics in living cells. [8][9][10] Current methods for rapidlym odulating cellular small molecules are based on optogenetic proteins, [11,12] chemical dimerizers [13,14] and photo-caged [15][16][17][18][19][20][21] or photo-switchable [19,[22][23][24] chemicalp robes. [8][9][10] Current methods for rapidlym odulating cellular small molecules are based on optogenetic proteins, [11,12] chemical dimerizers [13,14] and photo-caged [15][16][17][18][19][20][21] or photo-switchable [19,[22][23][24] chemicalp robes.…”

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“…We next assessed the GPCR ligandsa mong the new photocaged compounds (6,(8)(9)(10)(11)(12)(13)i nl ive cell fluorescencem icroscopy assays.W ef irst determined cellular uptake in HeLa Kyoto cells by fluorescencem icroscopy using the intrinsic fluorescence of the diethylamino-coumarin group as readout.A ll compounds proved to be membrane permeable, despite the fact that some molecules( 6, 10, 11, 12)a re intrinsicallyp ositively or negatively charged ( Figure 2B,F igure S4). While the compounds mostly exhibited the unspecific localization in cellular membranes typical for diethylamino-coumarin-caged molecules, overall fluorescencei ntensities varied significantly among compounds ( Figure S5).…”

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“…In Ta ble S1 for details) in HeLa Kyoto cells. We found that the caged fatty acids (7,8) can be used at all tested concentrations, whereas caged LPA (6), caged PAF( 10)a nd caged edelfosin (12)h ave narrower suitable concentration windows, while caged PGE 2 (13)w as found to be not suitable for leave-on experiments( Figure S8, see supplementary information for details). As ac ontrol we added the free ligandst oc ells not expressing the GPCRs and observed no PKCe recruitment to the plasma membrane or Ca 2 + transients ( Figure S7).…”

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A Coumarin Triflate Reagent Enables One‐Step Synthesis of Photo‐Caged Lipid Metabolites for Studying Cell Signaling

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Schuhmacher

Lohmann

et al. 2019

Chemistry A European J

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Photoreleaseo fc aged compoundsi sa mong the most powerful experimentala pproaches for studying cellularf unctions on fast timescales. However, its full potential has yett ob ee xploited, as the number of caged small molecules available for cell biological studies has been limited by synthetic challenges. Addressing this problem, as traightforward, one-step procedure fore fficiently synthesizing caged compounds was developed.A n in situ generated benzylic coumarin triflate reagent was used to specifically functionalize carboxylate and phosphate moieties in the presence of free hydroxy groups, generating variousc aged lipid metabolites, including a numbero fG PCR ligands. By combining the photo-caged ligandsw ith the respective receptors, an easily implementable experimental platform for the optical control and analysis of GPCR-mediated signal transduction in living cells wasd eveloped. Ultimately,t he described synthetic strategy allows rapid generation of photo-caged small moleculesa nd thus greatlyf acilitates the analysis of their biologicalr oles in live cell microscopy assays.

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Biophysical Approaches for Applying and Measuring Biological Forces

et al. 2021

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Over the past decades, increasing evidence has indicated that mechanical loads can regulate the morphogenesis, proliferation, migration, and apoptosis of living cells. Investigations of how cells sense mechanical stimuli or the mechanotransduction mechanism is an active field of biomaterials and biophysics. Gaining a further understanding of mechanical regulation and depicting the mechanotransduction network inside cells require advanced experimental techniques and new theories. In this review, the fundamental principles of various experimental approaches that have been developed to characterize various types and magnitudes of forces experienced at the cellular and subcellular levels are summarized. The broad applications of these techniques are introduced with an emphasis on the difficulties in implementing these techniques in special biological systems. The advantages and disadvantages of each technique are discussed, which can guide readers to choose the most suitable technique for their questions. A perspective on future directions in this field is also provided. It is anticipated that technical advancement can be a driving force for the development of mechanobiology.

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Mechanosensitive Fluorescent Probes to Image Membrane Tension in Mitochondria, Endoplasmic Reticulum, and Lysosomes

Cited by 177 publications

References 63 publications

A Chalcogen‐Bonding Cascade Switch for Planarizable Push–Pull Probes

A Chalcogen‐Bonding Cascade Switch for Planarizable Push–Pull Probes

A Coumarin Triflate Reagent Enables One‐Step Synthesis of Photo‐Caged Lipid Metabolites for Studying Cell Signaling

Biophysical Approaches for Applying and Measuring Biological Forces

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