4.8 Article

Thermodynamic Basis for Engineering High-Affinity, High-Specificity Binding-Induced DNA Clamp Nanoswitches

期刊

ACS NANO
卷 7, 期 12, 页码 10863-10869

出版社

AMER CHEMICAL SOC
DOI: 10.1021/nn404305e

关键词

clamp mechanism; triplex; DNA nanomachines; biomolecular switch; molecular beacons; specificity.; ligand-induced fit

资金

  1. Bill & Melinda Gates Foundation through the Grand Challenges Explorations [OPP1061203]
  2. International Research Staff Exchange Scheme (IRSES) grant under the Marie Curie Actions program
  3. NIH [R01EB007689]
  4. National Sciences and Engineering Research Council of Canada [436381-2013]
  5. Marie Curie Outgoing Fellowship (IOF) [298491]
  6. Canada-Italy innovation award
  7. Bill and Melinda Gates Foundation [OPP1061203] Funding Source: Bill and Melinda Gates Foundation

向作者/读者索取更多资源

Naturally occurring chemoreceptors almost invariably employ structure-switching mechanisms, an observation that has inspired the use of biomolecular switches in a wide range of artificial technologies in the areas of diagnostics, imaging, and synthetic biology. In one mechanism for generating such behavior, clamp-based switching, binding occurs via the clamplike embrace of two recognition elements onto a single target molecule. In addition to coupling recognition with a large conformational change, this mechanism offers a second advantage: it improves both affinity and specificity simultaneously. To explore the physics of such switches we have dissected here the thermodynamics of a clamp-switch that recognizes a target DNA sequence through both Watson Crick base pairing and triplex-forming Hoogsteen interactions. When compared to the equivalent linear DNA probe (which relies solely on Watson Crick interactions), the extra Hoogsteen interactions in the DNA clamp-switch increase the probe's affinity for its target by 0.29 +/-0.02 kcal/mol/base. The Hoogsteen interactions of the clamp-switch likewise provide an additional specificity check that increases the discrimination efficiency toward a single-base mismatch by 1.2+/-0.2 kcal/mol. This, in turn, leads to a 10-fold improvement in the width of the specificity window' of this probe relative to that of the equivalent linear probe. Given these attributes, clamp-switches should be of utility not only for sensing applications but also, in the specific field of DNA nanotechnology, for applications calling for a better control over the building of nanostructures and nanomachines.

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