Single-molecule FRET studies of the cooperative and non-cooperative binding kinetics of the bacteriophage T4 single-stranded DNA binding protein (gp32) to ssDNA lattices at replication fork junctions

Lee, Wonbae; Gillies, John P.; Jose, Davis; Israels, Brett; Hippel, Peter H. von; Marcus, Andrew H.

doi:10.1093/nar/gkw863

Cited by 12 publications

(33 citation statements)

References 43 publications

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“…The template strand contains a 15-nt poly(deoxythymidine) [p(dT) 15 ] sequence that can form an association complex with up to two cooperatively bound gp32 protein monomers at one time. Recently, Lee et al (15) showed that smFRET signals observed from this same p/t DNA construct in the presence of gp32 undergo intermittent protein-induced fluctuations, which reflect changes in the end to end distance of the ssDNA template caused by binding and dissociation of gp32 proteins.…”

Section: Significancementioning

confidence: 98%

Using microsecond single-molecule FRET to determine the assembly pathways of T4 ssDNA binding protein onto model DNA replication forks

Phelps

Israels

Jose

et al. 2017

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

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DNA replication is a core biological process that occurs in prokaryotic cells at high speeds (∼1 nucleotide residue added per millisecond) and with high fidelity (fewer than one misincorporation event per 10 nucleotide additions). The ssDNA binding protein [gene product 32 (gp32)] of the T4 bacteriophage is a central integrating component of the replication complex that must continuously bind to and unbind from transiently exposed template strands during DNA synthesis. We here report microsecond single-molecule FRET (smFRET) measurements on Cy3/Cy5-labeled primer-template (p/t) DNA constructs in the presence of gp32. These measurements probe the distance between Cy3/Cy5 fluorophores that label the ends of a short (15-nt) segment of ssDNA attached to a model p/t DNA construct and permit us to track the stochastic interconversion between various protein bound and unbound states. The length of the 15-nt ssDNA lattice is sufficient to accommodate up to two cooperatively bound gp32 proteins in either of two positions. We apply a unique multipoint time correlation function analysis to the microsecond-resolved smFRET data obtained to determine and compare the kinetics of various possible reaction pathways for the assembly of cooperatively bound gp32 protein onto ssDNA sequences located at the replication fork. The results of our analysis reveal the presence and translocation mechanisms of short-lived intermediate bound states that are likely to play a critical role in the assembly mechanisms of ssDNA binding proteins at replication forks and other ss duplex junctions.

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Section: Significancementioning

confidence: 98%

Using microsecond single-molecule FRET to determine the assembly pathways of T4 ssDNA binding protein onto model DNA replication forks

Phelps

Israels

Jose

et al. 2017

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

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“…As indicated above, we illustrate our approach using the macromolecular system studied by Lee et al , 8 in which a ssDNA template interacts with the T4 bacteriophage gp32 binding protein (see Fig. 1A).…”

Section: Conformational Transition Pathways and The Role Of Intermentioning

confidence: 99%

“…Experimentally, this requires making measurements at a higher time resolution than that used in the Lee et al study. 8 As the time resolution of a single-molecule fluorescence measurement approaches a few milliseconds, the signal will necessarily become too noisy to extract the state of the system through direct visualization of single-molecule trajectory data (e.g., by HMM analysis). Rather, we show below how equivalent information may be obtained through the application of the generalized concepts of TCFs.…”

Section: Conformational Transition Pathways and The Role Of Intermentioning

confidence: 99%

“…In a recent study from our laboratory, 8 smFRET experiments were employed to analyze the cooperative binding of the single-stranded (ss) DNA binding protein of the T4 bacteriophage DNA replication complex (gp32) to single-stranded segments of primer-template (p/t) DNA constructs of varying lengths and polarities. These constructs can serve as models of DNA replication forks.…”

Section: Introductionmentioning

confidence: 99%

“…As background, we note that gp32 protein molecules bind cooperatively and preferentially to ssDNA, with a binding site size of 7 nucleotide residues (nts, or DNA lattice positions) per gp32 molecule. 28 We have shown 8 that p/t DNA substrates with a ssDNA ‘tail’ region of 15 nts in length, which can cooperatively bind up to two gp32 proteins, can undergo stochastic fluctuations between 0-, 1- and 2-bound states (see Fig. 1A).…”

Section: Introductionmentioning

confidence: 99%

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Using Multiorder Time-Correlation Functions (TCFs) To Elucidate Biomolecular Reaction Pathways from Microsecond Single-Molecule Fluorescence Experiments

et al. 2016

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Recent advances in single-molecule fluorescence imaging have made it possible to perform measurements on microsecond time scales. Such experiments have the potential to reveal detailed information about conformational changes in biological macromolecules, including the reaction pathways and dynamics of the rearrangements involved in processes such as sequence-specific DNA ‘breathing’ and the assembly of protein-nucleic acid complexes. Because microsecond resolved single-molecule trajectories often involve ‘sparse’ data – i.e., they contain relatively few data points per unit time – they cannot be easily analyzed using the standard protocols that were developed for single-molecule experiments carried out with tens-of-millisecond time resolution and high ‘data density.’ We here describe a generalized approach, based on time correlation functions (TCFs), to obtain kinetic information from microsecond-resolved single-molecule fluorescence measurements. This approach can be used to identify short-lived intermediates that lie on reaction pathways connecting relatively long-lived reactant and product states. As a concrete illustration of the potential of this methodology for analyzing specific macromolecular systems, we accompany the theoretical presentation with a description of a specific biologically-relevant example drawn from studies of the reaction mechanisms of the assembly of the single-stranded DNA binding protein of the T4 bacteriophage replication complex onto a model DNA replication fork.

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DNA replication machinery: Insights from in vitro single-molecule approaches

Bocanegra

Płaza

Pulido

et al. 2021

Computational and Structural Biotechnology Journal

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Single-molecule FRET studies of the cooperative and non-cooperative binding kinetics of the bacteriophage T4 single-stranded DNA binding protein (gp32) to ssDNA lattices at replication fork junctions

Cited by 12 publications

References 43 publications

Using microsecond single-molecule FRET to determine the assembly pathways of T4 ssDNA binding protein onto model DNA replication forks

Using microsecond single-molecule FRET to determine the assembly pathways of T4 ssDNA binding protein onto model DNA replication forks

Using Multiorder Time-Correlation Functions (TCFs) To Elucidate Biomolecular Reaction Pathways from Microsecond Single-Molecule Fluorescence Experiments

DNA replication machinery: Insights from in vitro single-molecule approaches

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