Alessandro Valeri scite author profile

Two complementary methods in confocal single-molecule fluorescence spectroscopy are presented to analyze conformational dynamics by Forster resonance energy transfer (FRET) measurements considering simulated and experimental data. First, an extension of photon distribution analysis (PDA) is applied to characterize conformational exchange between two or more states via global analysis of the shape of FRET peaks for different time bins. PDA accurately predicts the shape of FRET efficiency histograms in the presence of FRET fluctuations, taking into account shot noise and background contributions. Dynamic-PDA quantitatively recovers FRET efficiencies of the interconverting states and relaxation times of dynamics on the time scale of the diffusion time t(d) (typically milliseconds), with a dynamic range of the method of about +/-1 order of magnitude with respect to t(d). Correction procedures are proposed to consider the factors limiting the accuracy of dynamic-PDA, such as brightness variations, shortening of the observation time due to diffusion, and a contribution of multimolecular events. Second, an analysis procedure for multiparameter fluorescence detection is presented, where intensity-derived FRET efficiency is correlated with the fluorescence lifetime of the donor quenched by FRET. If a maximum likelihood estimator is applied to compute a mean fluorescence lifetime of mixed states, one obtains a fluorescence weighted mean lifetime. Thus a mixed state is detected by a characteristic shift of the fluorescence lifetime, which becomes longer than that expected for a single species with the same intensity-derived FRET efficiency. Analysis tools for direct visual inspection of two-dimensional diagrams of FRET efficiency versus donor lifetime are presented for the cases of static and dynamic FRET. Finally these new techniques are compared with fluorescence correlation spectroscopy.

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Nucleosome disassembly intermediates characterized by single-molecule FRET

Gansen

Valeri

Hauger

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

173

201

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The nucleosome has a central role in the compaction of genomic DNA and the control of DNA accessibility for transcription and replication. To help understanding the mechanism of nucleosome opening and closing in these processes, we studied the disassembly of mononucleosomes by quantitative single-molecule FRET with high spatial resolution, using the SELEX-generated ''Widom 601'' positioning sequence labeled with donor and acceptor fluorophores. Reversible dissociation was induced by increasing NaCl concentration. At least 3 species with different FRET were identified and assigned to structures: (i) the most stable high-FRET species corresponding to the intact nucleosome, (ii) a less stable mid-FRET species that we attribute to a first intermediate with a partially unwrapped DNA and less histones, and (iii) a low-FRET species characterized by a very broad FRET distribution, representing highly unwrapped structures and free DNA formed at the expense of the other 2 species. Selective FCS analysis indicates that even in the low-FRET state, some histones are still bound to the DNA. The interdye distance of 54.0 Å measured for the high-FRET species corresponds to a compact conformation close to the known crystallographic structure. The coexistence and interconversion of these species is first demonstrated under non-invasive conditions. A geometric model of the DNA unwinding predicts the presence of the observed FRET species. The different structures of these species in the disassembly pathway map the energy landscape indicating major barriers for 10-bp and minor ones for 5-bp DNA unwinding steps.chromatin ͉ mononucleosomes ͉ structure T he nucleosome, the basic unit of genome compaction (1), consists of Ϸ2 turns of double-stranded DNA wound around a histone protein octamer. Its structure is known to a resolution of 1.9 Å (2). DNA sequence, chemical modifications and histone composition modulate gene activity through this structure.Central to nucleosomal function is its restructuring during processes that act on DNA, e.g., transcription or replication. Biochemical data indicate that nucleosome dissociation is temporary. Mechanisms for nucleosome unfolding, unwrapping or repositioning have been proposed (3), but so far none has been proven by direct physical evidence (e.g., detection of intermediate states). Here, we use single molecule Förster resonance energy transfer (FRET) to obtain quantitative structural information for elucidating such mechanisms.Bulk solution FRET is a proven tool for measuring average distances; nucleosome dynamics have been quantified by FRET between dyes attached to DNA and/or histone proteins (4-6). Analyzing FRET from single molecules (7, 8) can give detailed information on structural diversity; e.g., FRET on surfacetethered nucleosomes demonstrated spontaneous structure fluctuations (9, 10), whereas confocal spFRET experiments (11, 12) on freely diffusing single nucleosomes detected structural subpopulations under various conditions.The transit of a single molecule through the laser focus ...

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Single-cell absolute contact probability detection reveals chromosomes are organized by multiple low-frequency yet specific interactions

et al. 2017

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At the kilo- to megabase pair scales, eukaryotic genomes are partitioned into self-interacting modules or topologically associated domains (TADs) that associate to form nuclear compartments. Here, we combine high-content super-resolution microscopies with state-of-the-art DNA-labeling methods to reveal the variability in the multiscale organization of the Drosophila genome. We find that association frequencies within TADs and between TAD borders are below ~10%, independently of TAD size, epigenetic state, or cell type. Critically, despite this large heterogeneity, we are able to visualize nanometer-sized epigenetic domains at the single-cell level. In addition, absolute contact frequencies within and between TADs are to a large extent defined by genomic distance, higher-order chromosome architecture, and epigenetic identity. We propose that TADs and compartments are organized by multiple, small-frequency, yet specific interactions that are regulated by epigenetics and transcriptional state.

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