Imaging Cellular Dynamics with Spectral Relaxation Imaging Microscopy: Distinct Spectral Dynamics in Golgi Membranes of Living Cells

Lajevardipour, Alireza; Chon, James W. M.; Chattopadhyay, Amitabha; Clayton, Andrew H. A.

doi:10.1038/srep37038

Cited by 13 publications

(11 citation statements)

References 40 publications

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“…Moreover, a fluorescent sensor like Fl-GluBP may be useful for measuring synaptic viscosity. This may be through the relative fluorescence measurements of the binding and isomerization steps or by lifetime imaging as the lifetime is expected to increase if a singlet-exciplex intermediate is formed (28,29).…”

Section: Discussionmentioning

confidence: 99%

Kinetic Mechanisms of Fast Glutamate Sensing by Fluorescent Protein Probes

Coates

Kerruth

Helassa

et al. 2020

Biophysical Journal

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We have developed probes based on the bacterial periplasmic glutamate/aspartate binding protein with either an endogenously fluorescent protein or a synthetic fluorophore as the indicator of glutamate binding for studying the kinetic mechanism of glutamate binding. iGluSnFR variants termed iGlu h , iGlu m , and iGlu l cover a broad range of K d -s (5.8 mM and 2.1 and 50 mM, respectively), and a novel fluorescently labeled indicator, Fl-GluBP, has a K d of 9.7 mM. The fluorescence response kinetics of all the probes are consistent with a two-step mechanism involving ligand binding and isomerization either of the apo or the ligand-bound binding protein. Although the previously characterized ultrafast indicators iGlu u and iGlu f had monophasic fluorescence enhancement that occurred in the rate limiting isomerization step, the sensors described here all have biphasic binding kinetics with fluorescence increases occurring both in the glutamate binding and the isomerization steps. For iGlu m and iGlu l , the data indicate prebinding conformational change followed by ligand binding. In contrast, for iGlu h and Fl-GluBP, glutamate binding is followed by isomerization. Thus, the effects of structural heterogeneity introduced by single amino acid changes around the binding site on the kinetic path of interactions with glutamate are revealed. Remarkably, glutamate binding with a diffusionlimited rate constant to iGlu h and Fl-GluBP is detected for the first time, hinting at the underlying mechanism of the supremely rapid activation of the highly homologous a-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptor by glutamate binding.

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Section: Discussionmentioning

confidence: 99%

Kinetic Mechanisms of Fast Glutamate Sensing by Fluorescent Protein Probes

Coates

Kerruth

Helassa

et al. 2020

Biophysical Journal

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“… 11 to measure absolute concentrations of free and bound NADH in cells, using the FLIM-phasor method, a calibration sample of known concentration, and unmodulated light added to FLIM images. Among other micro-spectroscopy approaches using microenvironment sensitive spectral properties of fluorophores to characterize cellular processes in living cells, mention should be made of membrane studies using Laurdan 12 – 14 , di-4-ANEPPDHQ 15 , 16 , and NBD 17 fluorophores, using Generalized Polarization, GP , and the FLIM-phasor approaches.…”

Section: Introductionmentioning

confidence: 99%

Dynamic cellular maps of molecular species: Application to drug-target interactions

García

Losada

Sacristán

et al. 2018

Sci Rep

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The design of living cell studies aimed at deciphering the mechanism of action of drugs targeting proteins with multiple functions, expressed in a wide range of concentrations and cellular locations, is a real challenge. We recently showed that the antitumor drug plitidepsin (APL) localizes sufficiently close to the elongation factor eEF1A2 so as to suggest the formation of drug-protein complexes in living cells. Here we present an extension of our previous micro-spectroscopy study, that combines Generalized Polarization (GP) images, with the phasor approach and fluorescence lifetime imaging microscopy (FLIM), using a 7-aminocoumarin drug analog (APL*) as fluorescence tracer. Using the proposed methodology, we were able to follow in real time the formation and relative distribution of two sets of APL-target complexes in live cells, revealing two distinct patterns of behavior for HeLa-wt and APL resistant HeLa-APL-R cells. The information obtained may complement and facilitate the design of new experiments and the global interpretation of the results obtained with other biochemical and cell biology methods, as well as possibly opening new avenues of study to decipher the mechanism of action of new drugs.

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“…Incidentally, hydration dynamics at longer time scales (highlighted by a yellow bar in Figure ) could be influenced by biomembrane properties and coupled to membrane dynamics, possibly because of substantial temporal overlap in the two. In this context, we have recently reported faster solvent relaxation in the Golgi membrane of live cells relative to the plasma membrane, utilizing a fluorescence-based spectral relaxation imaging approach . It must be noted here that the temporal aspects of hydration dynamics discussed above, particularly that of membrane-coupled hydration dynamics, is undergoing a rapid conceptual evolution at present.…”

mentioning

confidence: 87%

Hydration Dynamics in Biological Membranes: Emerging Applications of Terahertz Spectroscopy

Pal

Chattopadhyay

2021

J. Phys. Chem. Lett.

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Water drives the spontaneous self-assembly of lipids and proteins into quasi two-dimensional biological membranes that act as catalytic scaffolds for numerous processes central to life. However, the functional relevance of hydration in membrane biology is only beginning to be addressed, predominantly because of challenges associated with direct measurements of hydration microstructure and dynamics in a biological milieu. Our recent work on the novel interplay of membrane electrostatics and crowding in shaping membrane hydration dynamics utilizing terahertz (THz) spectroscopy represents an important step in this context. In this Perspective, we provide a glimpse into the ever-broadening functional landscape of hydration dynamics in biological membranes in the backdrop of the unique physical chemistry of water molecules. We further highlight the immense (and largely untapped) potential of the THz toolbox in addressing contemporary problems in membrane biology, while emphasizing the adaptability of the analytical framework reported recently by us to such studies.

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Imaging Cellular Dynamics with Spectral Relaxation Imaging Microscopy: Distinct Spectral Dynamics in Golgi Membranes of Living Cells

Cited by 13 publications

References 40 publications

Kinetic Mechanisms of Fast Glutamate Sensing by Fluorescent Protein Probes

Kinetic Mechanisms of Fast Glutamate Sensing by Fluorescent Protein Probes

Dynamic cellular maps of molecular species: Application to drug-target interactions

Hydration Dynamics in Biological Membranes: Emerging Applications of Terahertz Spectroscopy

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