Fast Folding of RNA Pseudoknots Initiated by Laser Temperature-Jump

Narayanan, Ranjani; Velmurugu, Yogambigai; Kuznetsov, Serguei V.; Ansari, Anjum

doi:10.1021/ja205737v

Cited by 25 publications

(46 citation statements)

References 69 publications

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“…together with probes such as tryptophans and fluorescent nucleotide analogs, has led to the characterization of otherwise unresolved conformational dynamics during protein folding (42)(43)(44)(45), RNA folding (46), and protein-DNA (47-49) and protein-RNA (50) interactions.…”

Section: Significancementioning

confidence: 99%

Twist-open mechanism of DNA damage recognition by the Rad4/XPC nucleotide excision repair complex

Velmurugu

Chen

Sevilla

et al. 2016

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

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125

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DNA damage repair starts with the recognition of damaged sites from predominantly normal DNA. In eukaryotes, diverse DNA lesions from environmental sources are recognized by the xeroderma pigmentosum C (XPC) nucleotide excision repair complex. Studies of Rad4 (radiation-sensitive 4; yeast XPC ortholog) showed that Rad4 "opens" up damaged DNA by inserting a β-hairpin into the duplex and flipping out two damage-containing nucleotide pairs. However, this DNA lesion "opening" is slow (~5-10 ms) compared with typical submillisecond residence times per base pair site reported for various DNA-binding proteins during 1D diffusion on DNA. To address the mystery as to how Rad4 pauses to recognize lesions during diffusional search, we examine conformational dynamics along the lesion recognition trajectory using temperaturejump spectroscopy. Besides identifying the~10-ms step as the ratelimiting bottleneck towards opening specific DNA site, we uncover an earlier~100-to 500-μs step that we assign to nonspecific deformation (unwinding/"twisting") of DNA by Rad4. The β-hairpin is not required to unwind or to overcome the bottleneck but is essential for full nucleotide-flipping. We propose that Rad4 recognizes lesions in a step-wise "twist-open" mechanism, in which preliminary twisting represents Rad4 interconverting between search and interrogation modes. Through such conformational switches compatible with rapid diffusion on DNA, Rad4 may stall preferentially at a lesion site, offering time to open DNA. This study represents the first direct observation, to our knowledge, of dynamical DNA distortions during search/interrogation beyond base pair breathing. Submillisecond interrogation with preferential stalling at cognate sites may be common to various DNA-binding proteins.DNA damage recognition | time-resolved fluorescence spectroscopy | temperature-jump perturbation | DNA unwinding dynamics | xeroderma pigmentosum E ssential genetic mechanisms, such as replication, transcription, recombination, and repair, all require recognition of specific DNA sequences or structures by specialized proteins. How DNA-binding proteins search for and identify their target sites embedded in a vast excess of nontarget sites, especially if using only thermal energy, is a fundamental question in biology. Several lines of evidence indicate that proteins use some combination of 3D diffusion in the bulk solution and 1D diffusion while nonspecifically bound to DNA, and use this "facilitated diffusion" as a means to search efficiently in genomic DNA for their targets (1-7). Direct observations of proteins diffusing on nonspecific DNA have revealed residence times per base pair site ranging from 50 ns to 300 μs (7-13). On the other end, highresolution structures and thermodynamic studies on a wide range of specific protein-DNA complexes have revealed significant distortions in otherwise B-form DNA duplex structures and concerted rearrangements in the bound protein to accommodate the deformed DNA; this "induced-fit" mechanism has emerged as a general pr...

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Section: Significancementioning

confidence: 99%

Twist-open mechanism of DNA damage recognition by the Rad4/XPC nucleotide excision repair complex

Velmurugu

Chen

Sevilla

et al. 2016

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

Self Cite

125

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“…Our observation of multiple intermediates in pseudoknot folding agrees with numerous previous observations and predictions including the simple model of Ansari et al . based on laser T-jump experiments (32) and the folding pathways predicted from coarse-grained simulations by Thirumalai et al . (33).…”

Section: Resultsmentioning

confidence: 99%

“…While the M 1 through M 3 misfolds might easily be clustered or classified into a larger number of misfolded states, our analysis has emphasized macroscopically measurable structural characteristics and both M 2 and M 3 represent misfolds predicted by the statistical mechanical model of Ansari et al . (32). …”

Section: Resultsmentioning

confidence: 99%

Ensemble simulations: folding, unfolding and misfolding of a high-efficiency frameshifting RNA pseudoknot

et al. 2017

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Massive all-atom molecular dynamics simulations were conducted across a distributed computing network to study the folding, unfolding, misfolding and conformational plasticity of the high-efficiency frameshifting double mutant of the 26 nt potato leaf roll virus RNA pseudoknot. Our robust sampling, which included over 40 starting structures spanning the spectrum from the extended unfolded state to the native fold, yielded nearly 120 μs of cumulative sampling time. Conformational microstate transitions on the 1.0 ns to 10.0 μs timescales were observed, with post-equilibration sampling providing detailed representations of the conformational free energy landscape and the complex folding mechanism inherent to the pseudoknot motif. Herein, we identify and characterize two alternative native structures, three intermediate states, and numerous misfolded states, the latter of which have not previously been characterized via atomistic simulation techniques. While in line with previous thermodynamics-based models of a general RNA folding mechanism, our observations indicate that stem-strand-sequence-separation may serve as an alternative predictor of the order of stem formation during pseudoknot folding. Our results contradict a model of frameshifting based on structural rigidity and resistance to mechanical unfolding, and instead strongly support more recent studies in which conformational plasticity is identified as a determining factor in frameshifting efficiency.

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“…Indeed, even simple RNA hairpins and pseudoknots have complex folding kinetics. [30,[34][35][36][37] However, the similar themes imply that the same formalism and concepts from protein folding can serve as a basis for the study of nucleic acid folding mechanisms. [32,38] 3 Bottom-Up and Top-Down Approaches for Biomolecular MD Simulations MD simulations continue to be an indispensable tool for the study of biomolecular folding and assembly mechanisms.…”

Section: Nucleic Acid Folding Energy Landscapesmentioning

confidence: 99%

“…[30] The folding times predicted by the TIS model were remarkably similar to the relaxation times measured by Ansari and coworkers in a subsequent laser temperature-jump perturbation study. [37] Inspired by interrupted multiple ion-jump single-molecule experiments, [67] Biyun et al developed novel ion-concentration induced jump TIS model MD simulations by abruptly changing the ion concentration in the DebyeÀHückel potential. [36] Very recently, Li et al performed TIS model simulations of four different tRNA molecules of similar length and tertiary structure but different sequence.…”

Section: Atomistic Empirical Force Field MD Simulations Of Rna Foldingmentioning

confidence: 99%

Coarse‐Grained and Atomistic MD Simulations of RNA and DNA Folding

Leuchter

Green

Gilyard

et al. 2014

Israel Journal of Chemistry

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Although the main features of the protein folding problem are coming into clearer focus, the microscopic viewpoint of nucleic acid folding mechanisms is only just beginning to be addressed. Experiments, theory, and simulations are pointing to complex thermodynamic and kinetic mechanisms. As is the case for proteins, molecular dynamics (MD) simulations continue to be indispensable tools for providing a molecular basis for nucleic acid folding mechanisms. In this review, we provide an overview of biomolecular folding mechanisms focusing on nucleic acids. We outline the important interactions that are likely to be the main determinants of nucleic acid folding energy landscapes. We discuss recent MD simulation studies of empirical force field and Go‐type MD simulations of RNA and DNA folding mechanisms to outline recent successes and the theoretical and computational challenges that lie ahead.

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Fast Folding of RNA Pseudoknots Initiated by Laser Temperature-Jump

Cited by 25 publications

References 69 publications

Twist-open mechanism of DNA damage recognition by the Rad4/XPC nucleotide excision repair complex

Twist-open mechanism of DNA damage recognition by the Rad4/XPC nucleotide excision repair complex

Ensemble simulations: folding, unfolding and misfolding of a high-efficiency frameshifting RNA pseudoknot

Coarse‐Grained and Atomistic MD Simulations of RNA and DNA Folding

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