Long Lifetime of Hydrogen-Bonded DNA Basepairs by Force Spectroscopy

Fuhrmann, Alexander; Getfert, Sebastian; Fu, Qiang; Reimann, Peter; Lindsay, Stuart; Ros, Robert

doi:10.1016/j.bpj.2012.04.006

Cited by 18 publications

(18 citation statements)

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“…This is in agreement with our measurements of the lifetime of similar complexes using atomic force microscopy, where we have observed that the zero-force lifetime of hydrogen-bonded complexes tethered in a nanogap is on the order of seconds. 12, 19 Thus, recognition-tunneling may also provide a tool for slowing DNA transport in a nanopore reader.…”

Section: 0 Results and Discussionmentioning

confidence: 99%

“…The off-rates are slow (corresponding to lifetimes of seconds) consistent with AFM measurements of the lifetimes of hydrogen-bonded complexes in a nanogap. 19, 12 This behavior has recently been explained as a consequence of the bond confinement in the gap. 21 The on-rates are fast, probably too fast to be measured with the techniques used here, but certainly consistent with DNA sequencing speeds of many tens of bases per second.…”

Section: 0 Conclusionmentioning

confidence: 92%

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Chemical recognition and binding kinetics in a functionalized tunnel junction

et al. 2012

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4(5)-(2-mercaptoethyl)-1H-imidazole-2-carboxamide is a molecule that has multiple hydrogen bonding sites and a short flexible linker. When tethered to a pair of electrodes, it traps target molecules in a tunnel junction. Surprisingly large recognition-tunneling signals are generated for all naturally occurring DNA bases A, C, G,T, and 5-methyl-Cytosine. Tunnel current spikes are stochastic and broadly distributed, but characteristic enough so that individual bases can be identified as a tunneling probe is scanned over DNA oligomers. Each base yields a recognizable burst of signal, the duration of which is controlled entirely by the probe speed, down to speeds of 1 nm/s, implying a maximum off-rate of 3 s-1 for the recognition complex. The same measurements yield a lower bound on the on-rate of ~1 M-1s-1. Despite the stochastic nature of the signals, an optimized multi-parameter fit allows base-calling from a single signal peak with an accuracy that can exceed 80% when a single type of nucleotide is present in the junction, meaning that recognition-tunneling is capable of true single-molecule analysis. The accuracy increases to 95% when multiple spikes in a signal cluster are analyzed.

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Section: 0 Results and Discussionmentioning

confidence: 99%

Section: 0 Conclusionmentioning

confidence: 92%

Chemical recognition and binding kinetics in a functionalized tunnel junction

et al. 2012

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“…Similarly, AFM force spectroscopy experiments show that the lifetime of single base-pairs formed via either 2 or 3 H-bonds is B2 and 4 s, respectively 40 . Furthermore, these experiments show that H-bonds exhibit lifetimes larger than 0.1 s even in the presence of 40-60 pN load 40 .…”

Section: Article Nature Communications | Doi: 101038/ncomms4941mentioning

confidence: 92%

Resolving the molecular mechanism of cadherin catch bond formation

et al. 2014

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Classical cadherin Ca 2 þ -dependent cell-cell adhesion proteins play key roles in embryogenesis and in maintaining tissue integrity. Cadherins mediate robust adhesion by binding in multiple conformations. One of these adhesive states, called an X-dimer, forms catch bonds that strengthen and become longer lived in the presence of mechanical force. Here we use single-molecule force-clamp spectroscopy with an atomic force microscope along with molecular dynamics and steered molecular dynamics simulations to resolve the molecular mechanisms underlying catch bond formation and the role of Ca 2 þ ions in this process. Our data suggest that tensile force bends the cadherin extracellular region such that they form long-lived, force-induced hydrogen bonds that lock X-dimers into tighter contact. When Ca 2 þ concentration is decreased, fewer de novo hydrogen bonds are formed and catch bond formation is eliminated.

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“…In order to eliminate hidden multiple unbinding events from visibly indistinguishable single unbinding events, we followed a protocol used for identifying the heterogeneity in chemical bonds or hidden multiple bonds as described previously (Fuhrmann et al, 2012). After eliminating all hidden multiple events, the forces were plotted as a histogram for each retracting velocity with bin width calculated according to a statistical method (Scott, 1979).…”

Section: Single Molecule Dynamic Force Spectroscopy Experimentsmentioning

confidence: 99%

Different roles of cadherins in the assembly and structural integrity of the desmosome complex

Lowndes

Rakshit

Shafraz

et al. 2014

Journal of Cell Science

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Adhesion between cells is established by the formation of specialized intercellular junctional complexes, such as desmosomes. Desmosomes contain isoforms of two members of the cadherin superfamily of cell adhesion proteins, desmocollins (Dsc) and desmogleins (Dsg), but their combinatorial roles in desmosome assembly are not understood. To uncouple desmosome assembly from other cell-cell adhesion complexes, we used micro-patterned substrates of Dsc2aFc and/or Dsg2Fc and collagen IV; we show that Dsc2aFc, but not Dsg2Fc, was necessary and sufficient to recruit desmosome-specific desmoplakin into desmosome puncta and produce strong adhesive binding. Single-molecule force spectroscopy showed that monomeric Dsc2a, but not Dsg2, formed Ca 2+ -dependent homophilic bonds, and that Dsg2 formed Ca 2+ -independent heterophilic bonds with Dsc2a. A W2A mutation in Dsc2a inhibited Ca 2+ -dependent homophilic binding, similar to classical cadherins, and Dsc2aW2A, but not Dsg2W2A, was excluded from desmosomes in MDCK cells. These results indicate that Dsc2a, but not Dsg2, is required for desmosome assembly through homophilic Ca 2+ -and W2-dependent binding, and that Dsg2 might be involved later in regulating a switch to Ca 2+ -independent adhesion in mature desmosomes.

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Long Lifetime of Hydrogen-Bonded DNA Basepairs by Force Spectroscopy

Cited by 18 publications

References 50 publications

Chemical recognition and binding kinetics in a functionalized tunnel junction

Chemical recognition and binding kinetics in a functionalized tunnel junction

Resolving the molecular mechanism of cadherin catch bond formation

Different roles of cadherins in the assembly and structural integrity of the desmosome complex

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