Mechanistic Insights From Single-Molecule Studies of Repair of Double Strand Breaks

Kong, Muwen; Greene, Eric C.

doi:10.3389/fcell.2021.745311

Cited by 7 publications

(3 citation statements)

References 199 publications

(259 reference statements)

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“…Watching DNA-binding proteins interact with DNA substrates in real-time at the single-molecule level illuminates how proteins detect and bind their targets at extraordinary detail. Key information about binding stoichiometry, order of assembly and disassembly, and how proteins diffuse to find their DNA targets are gained through single-molecule analysis (1)(2)(3). Various imaging techniques and optical platforms have been employed to resolve fluorescent proteins to the single-molecule level, but most of these techniques cluster into two broad categories -studies performed with purified proteins with defined conditions (1,4,5) or studies performed in living cells (6)(7)(8).…”

Section: Introductionmentioning

confidence: 99%

Single-molecule analysis of DNA-binding proteins from nuclear extracts (SMADNE)

Schaich

Schnable

Kumar

et al. 2023

Nucleic Acids Research

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Single-molecule characterization of protein–DNA dynamics provides unprecedented mechanistic details about numerous nuclear processes. Here, we describe a new method that rapidly generates single-molecule information with fluorescently tagged proteins isolated from nuclear extracts of human cells. We demonstrated the wide applicability of this novel technique on undamaged DNA and three forms of DNA damage using seven native DNA repair proteins and two structural variants, including: poly(ADP-ribose) polymerase (PARP1), heterodimeric ultraviolet-damaged DNA-binding protein (UV-DDB), and 8-oxoguanine glycosylase 1 (OGG1). We found that PARP1 binding to DNA nicks is altered by tension, and that UV-DDB did not act as an obligate heterodimer of DDB1 and DDB2 on UV-irradiated DNA. UV-DDB bound to UV photoproducts with an average lifetime of 39 seconds (corrected for photobleaching, τc), whereas binding lifetimes to 8-oxoG adducts were < 1 second. Catalytically inactive OGG1 variant K249Q bound oxidative damage 23-fold longer than WT OGG1, at 47 and 2.0 s, respectively. By measuring three fluorescent colors simultaneously, we also characterized the assembly and disassembly kinetics of UV-DDB and OGG1 complexes on DNA. Hence, the SMADNE technique represents a novel, scalable, and universal method to obtain single-molecule mechanistic insights into key protein–DNA interactions in an environment containing physiologically-relevant nuclear proteins.

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Section: Introductionmentioning

confidence: 99%

Single-molecule analysis of DNA-binding proteins from nuclear extracts (SMADNE)

Schaich

Schnable

Kumar

et al. 2023

Nucleic Acids Research

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show abstract

“…A central component of any single-molecule experiment designed to understand the mechanism of action of proteins that interact with DNA is the DNA construct itself (Bocanegra, Plaza, Pulido, & Ibarra, 2021;Dulin, Lipfert, Moolman, & Dekker, 2013;Kong & Greene, 2021;Ordu, Lusser, & Dekker, 2016;Spinks, Spenkelink, Dixon, & van Oijen, 2021;Yodh, Schlierf, & Ha, 2010). Moreover, the production of dedicated DNA constructs has been critical to unveil their mechanical properties and how these modulate the activity of processing enzymes; information that is hardly achievable using bulk methods (Basu, Bobrovnikov, & Ha, 2021;Brahmachari & Marko, 2018;Bustamante, Bryant, & Smith, 2003;Camunas-Soler, Ribezzi-Crivellari, & Ritort, 2016;Marin-Gonzalez, Vilhena, Perez, & Moreno-Herrero, 2021).…”

Section:  1 Introductionmentioning

confidence: 99%

Long DNA constructs to study helicases and nucleic acid translocases using optical tweezers

Aicart-Ramos

Hormeño

Wilkinson

et al. 2022

Helicase Enzymes Part B

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“…Watching DNA-binding proteins interact with DNA substrates in real-time at the single-molecule level illuminates how proteins detect and bind their targets at extraordinary detail. Key information about binding stoichiometry, order of assembly and disassembly, and how proteins diffuse to find their DNA targets are gained through single molecule analysis [1][2][3] . Various imaging techniques and optical platforms have been employed to resolve fluorescent proteins to the single-molecule level, but most of these techniques cluster into two broad categories -studies performed with purified proteins with defined conditions [4][5][6] or studies performed in living cells [7][8][9] .…”

Section: Introductionmentioning

confidence: 99%

Single-Molecule Analysis of DNA-binding proteins from Nuclear Extracts (SMADNE)

Schaich

Schnable

Kumar

et al. 2022

Preprint

View full text Add to dashboard Cite

Single-molecule characterization of protein-DNA dynamics provides unprecedented mechanistic details about numerous nuclear processes. Here, we describe a new method that rapidly generates single-molecule information for fluorescently tagged proteins isolated from nuclear extracts of human cells. This approach determines binding lifetimes (koff), events per second (~kon), positional dependence (specificity), and characterizes 1D diffusion along DNA. We demonstrated the wide applicability of this approach on three forms of DNA damage using seven native DNA repair proteins and two structural variants, including: poly(ADP-ribose) polymerase (PARP1), heterodimeric ultraviolet-damaged DNA-binding protein (UV-DDB), xeroderma pigmentosum complementation group C protein (XPC), and 8-oxoguanine glycosylase 1 (OGG1). By measuring multiple fluorescent colors simultaneously, we additionally characterized the assembly and disassembly kinetics of multi-protein complexes on DNA. Thus, Single-Molecule Analysis of DNA-binding proteins from Nuclear Extracts (SMADNE) provides new insights about damage recognition and represents a universal technique that can be used to rapidly characterize numerous protein-DNA interactions.

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Mechanistic Insights From Single-Molecule Studies of Repair of Double Strand Breaks

Cited by 7 publications

References 199 publications

Single-molecule analysis of DNA-binding proteins from nuclear extracts (SMADNE)

Single-molecule analysis of DNA-binding proteins from nuclear extracts (SMADNE)

Long DNA constructs to study helicases and nucleic acid translocases using optical tweezers

Single-Molecule Analysis of DNA-binding proteins from Nuclear Extracts (SMADNE)

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