Multiparameter single-molecule fluorescence spectroscopy reveals heterogeneity of HIV-1 reverse transcriptase:primer/template complexes

Rothwell, Paul J.; Berger, Sylvia; Kensch, Oliver; Felekyan, Suren; Antonik, Matthew; Wöhrl, Birgitta M.; Restle, Tobias; Goody, Roger S.; Seidel, Claus A. M.

doi:10.1073/pnas.0434003100

Cited by 217 publications

(257 citation statements)

References 27 publications

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“…Additionally, the analysis provides the variance of the bin heights as (28) Unfortunately, experimental PRH do not necessarily result in posterior probability having a maximum (that is, the resulting LPP can either be monotically increasing or exhibit only a local maximum). This results from the discrete nature of its rational values.…”

Section: Discussionmentioning

confidence: 99%

Shot-Noise Limited Single-Molecule FRET Histograms: Comparison between Theory and Experiments

et al. 2006

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We describe a simple approach and present a straightforward numerical algorithm to compute the best fit shot-noise limited proximity ratio histogram (PRH) in single-molecule fluorescence resonant energy transfer diffusion experiments. The key ingredient is the use of the experimental burst size distribution, as obtained after burst search through the photon data streams. We show how the use of an alternated laser excitation scheme and a correspondingly optimized burst search algorithm eliminates several potential artifacts affecting the calculation of the best fit shot-noise limited PRH. This algorithm is tested extensively on simulations and simple experimental systems. We find that dsDNA data exhibit a wider PRH than expected from shot noise only and hypothetically account for it by assuming a small Gaussian distribution of distances with an average standard deviation of 1.6 Å. Finally, we briefly mention the results of a future publication and illustrate them with a simple two-state model system (DNA hairpin), for which the kinetic transition rates between the open and closed conformations are extracted.

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Section: Discussionmentioning

confidence: 99%

Shot-Noise Limited Single-Molecule FRET Histograms: Comparison between Theory and Experiments

et al. 2006

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“…Using this subspecies of molecules, the direct excitation coefficient a can be calculated from the ratio of the background corrected number of photons in the acceptor channel after donor excitation to the background corrected number of photons in the acceptor channel after acceptor excitation [Eq. (27)]:…”

Section: Optical Alignmentmentioning

confidence: 99%

“…[25,26] The lifetime and anisotropy information can be utilized to extract quantitative distances from spFRET experiments. [27] Another important development that allows separation of low-FRET complexes from complexes missing a photoactive acceptor molecule is alternating laser excitation (ALEX) introduced by Kapanidis and coworkers. In ALEX experiments, the donor and acceptor dyes are excited alternately on the ms timescale using continuous-wave lasers alternated by an electro-optical modulator.…”

Section: Introductionmentioning

confidence: 99%

Combining MFD and PIE for Accurate Single‐Pair Förster Resonance Energy Transfer Measurements

et al. 2012

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“…Static FRET measurements have also been used previously to characterize the pre-translocation and post-translocation states of RT on a DNA duplex 28 . Because RT accommodates 19-22 base pairs of nucleic-acid duplex within its primer-template-binding cleft 19,22,29 (Fig.…”

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confidence: 99%

Dynamic binding orientations direct activity of HIV reverse transcriptase

Abbondanzieri¹,

Bokinsky²,

Rausch

et al. 2008

Nature

171

216

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The reverse transcriptase of human immunodeficiency virus (HIV) catalyses a series of reactions to convert the single-stranded RNA genome of HIV into double-stranded DNA for host-cell integration. This task requires the reverse transcriptase to discriminate a variety of nucleic-acid substrates such that active sites of the enzyme are correctly positioned to support one of three catalytic functions: RNA-directed DNA synthesis, DNA-directed DNA synthesis and DNA-directed RNA hydrolysis. However, the mechanism by which substrates regulate reverse transcriptase activities remains unclear. Here we report distinct orientational dynamics of reverse transcriptase observed on different substrates with a single-molecule assay. The enzyme adopted opposite binding orientations on duplexes containing DNA or RNA primers, directing its DNA synthesis or RNA hydrolysis activity, respectively. On duplexes containing the unique polypurine RNA primers for plus-strand DNA synthesis, the enzyme can rapidly switch between the two orientations. The switching kinetics were regulated by cognate nucleotides and non-nucleoside reverse transcriptase inhibitors, a major class of anti-HIV drugs. These results indicate that the activities of reverse transcriptase are determined by its binding orientation on substrates.Virtually all RNA-processing and DNA-processing enzymes show selectivity for backbone compositions or base sequences of their nucleic-acid substrates. This substrate selectivity is especially crucial for the HIV-1 reverse transcriptase (RT), which binds and discriminates between a variety of nucleic-acid duplexes for distinct catalytic functions 1,2 . RT is a heterodimer consisting of a p51 and a p66 subunit, the latter of which contains catalytically active DNA polymerase and RNase H domains 3,4 , catalysing a complex, multi-step reaction to convert the single-stranded RNA genome into double-stranded DNA 1,2 . First, RT uses the viral RNA genome as a template and a host-cell transfer RNA as a primer to synthesize a minus-strand DNA, producing an RNA-DNA hybrid [5][6][7] . This duplex becomes the substrate of the RNase H domain of RT, which cleaves the RNA strand at numerous points, leaving behind short RNA segments hybridized to the nascent DNA [8][9][10] . Among these RNAs, two specific purine-rich sequences, known as the polypurine tracts (PPTs), serve as unique primers to initiate the synthesis of plus-strand DNA 11-13 , thereby creating the double-stranded DNA viral genome. Specific cleavage by RNase H then removes the PPT primers and exposes the integration sequence to facilitate the insertion of the viral DNA into the host chromosome 14 . Inappropriate initiation of synthesis of the plus-strand DNA at other RNA segments prevents integration 2,15 . RT must therefore obey the following primer-selection rules: first, DNA primers readily engage the polymerase activity of RT; second, generic RNA primers are not efficiently extended by RT but readily engage the RNase H activity of RT when annealed with DNA; third, the PPT RNA ca...

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Multiparameter single-molecule fluorescence spectroscopy reveals heterogeneity of HIV-1 reverse transcriptase:primer/template complexes

Cited by 217 publications

References 27 publications

Shot-Noise Limited Single-Molecule FRET Histograms: Comparison between Theory and Experiments

Shot-Noise Limited Single-Molecule FRET Histograms: Comparison between Theory and Experiments

Combining MFD and PIE for Accurate Single‐Pair Förster Resonance Energy Transfer Measurements

Dynamic binding orientations direct activity of HIV reverse transcriptase

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