Submolecular dissection reveals strong and specific binding of polyamide–pyridostatin conjugates to human telomere interface

Mandal, Shankar; Kawamoto, Yusuke; Yue, Zhizhou; Hashiya, Kaori; Cui, Yunxi; Bando, Toshikazu; Pandey, Shankar; Hoque, Mohammed Enamul; Hossain, Mohammad Akter; Sugiyama, Hiroshi; Mao, Hanbin

doi:10.1093/nar/gkz135

Cited by 20 publications

(6 citation statements)

References 59 publications

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“…Dibenzocyclooctyne-N-hydroxysuccinimidyl ester was purchased from Sigma Aldrich. Azide modified pyridostatin was prepared as described in literature ( 13 ). The streptavidin or anti-digoxigenin coated polystyrene beads were purchased from Spherotech.…”

Section: Methodsmentioning

confidence: 99%

Dissection of nanoconfinement and proximity effects on the binding events in DNA origami nanocavity

Jonchhe

Pandey

Beneze

et al. 2022

Nucleic Acids Research

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Both ligand binding and nanocavity can increase the stability of a biomolecular structure. Using mechanical unfolding in optical tweezers, here we found that a DNA origami nanobowl drastically increased the stability of a human telomeric G-quadruplex bound with a pyridostatin (PDS) ligand. Such a stability change is equivalent to >4 orders of magnitude increase (upper limit) in binding affinity (Kd: 490 nM → 10 pM (lower limit)). Since confined space can assist the binding through a proximity effect between the ligand-receptor pair and a nanoconfinement effect that is mediated by water molecules, we named such a binding as mechanochemical binding. After minimizing the proximity effect by using PDS that can enter or leave the DNA nanobowl freely, we attributed the increased affinity to the nanoconfinement effect (22%) and the proximity effect (78%). This represents the first quantification to dissect the effects of proximity and nanoconfinement on binding events in nanocavities. We anticipate these DNA nanoassemblies can deliver both chemical (i.e. ligand) and mechanical (i.e. nanocavity) milieus to facilitate robust mechanochemical binding in various biological systems.

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Section: Methodsmentioning

confidence: 99%

Dissection of nanoconfinement and proximity effects on the binding events in DNA origami nanocavity

Jonchhe

Pandey

Beneze

et al. 2022

Nucleic Acids Research

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“…We found that average mechanical stability of (dA) 21 strands adsorbed on these three AuNPs is ∼40 pN. This value is significantly higher than the stall force of DNA/RNA polymerases. − Therefore, similar to the G-quadruplex that may serve as a mechanical block , to DNA replication or RNA transcription processes, the AuNP-poly(dA) may also serve similar functions, given that there are plenty of poly(dA) segments in genomes of many species. − This potential function further expands the applicability of AuNP in biomedicines. This approach of determining the mechanical stability of DNA corona phase on nanoparticles can also be extended to other materials such as carbon nanotubes which are of growing interest in recent years .…”

Section: Resultsmentioning

confidence: 89%

“…This value is significantly higher than the stall force of DNA/RNA polymerases. 37−39 Therefore, similar to the G-quadruplex that may serve as a mechanical block 47,48 to DNA replication or RNA transcription processes, the AuNP-poly(dA) may also serve similar functions, given that there are plenty of poly(dA) segments in genomes of many species. 41−43 This potential function further expands the applicability of AuNP in biomedicines.…”

Section: ■ Results and Discussionmentioning

confidence: 99%

Mechanical Stability of DNA Corona Phase on Gold Nanospheres

et al. 2022

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Noncovalent adsorption of biopolymers on the surface of gold nanoparticles (AuNPs) forms a corona phase that drastically diversify AuNP functions. However, mechanical stabilities of such corona phase are still obscure, hindering the application of biopolymer-coated AuNPs. Here, using optical tweezers, we have observed, for the first time, that DNA corona phase adsorbed on a 5 nm AuNP via two (dA)21 strands in proximity can withstand an average desorption force of 40 pN, which is higher than the stall force of DNA/RNA polymerases. This suggests a new role for AuNPs to modulate replications or transcriptions after binding to prevalent poly(dA) segments in eukaryotic genomes. We have also revealed that with increasing AuNP size (1.8–10 nm), DNA corona becomes harder to remove, likely due to the larger surfaces and flatter facets on bigger AuNPs. These findings provide guidance to design AuNP corona that can withstand harsh environments for biological and materials applications.

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“…The binding of PDS to telomere G4s resulted in the shift of the unfolding force peak of G4s in K + solution from ~21 pN to~41 pN, suggesting a strong reduction in unfolding rate. Since then, the applications of force–spectroscopy techniques further enable the characterization of interactions between quadruplexes and quadruplexes [ 108 ], small ligands and quadruplexes [ 52 , 109 , 110 , 111 , 112 ], proteins and quadruplexes [ 63 , 64 , 65 ], and study on factors that affect the folding/unfolding dynamics of G4s, including molecular crowding [ 113 ], force at different directions [ 84 , 110 ], nanoconfinement [ 91 , 92 , 93 ], DNA superhelicity [ 88 ], and RNA transcripts [ 114 ]. The force spectroscopy has also been used to study the folding/unfolding dynamics of other four strands nucleic acid structures i-motif, which are located at the opposite strand of G4s [ 115 , 116 ], and the molecular switch between G4s and i-motif [ 117 ].…”

Section: Single-molecule Force Spectroscopy For the Investigation Of G-quadruplexesmentioning

confidence: 99%

Characterization of G-Quadruplexes Folding/Unfolding Dynamics and Interactions with Proteins from Single-Molecule Force Spectroscopy

2021

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G-quadruplexes (G4s) are stable secondary nucleic acid structures that play crucial roles in many fundamental biological processes. The folding/unfolding dynamics of G4 structures are associated with the replication and transcription regulation functions of G4s. However, many DNA G4 sequences can adopt a variety of topologies and have complex folding/unfolding dynamics. Determining the dynamics of G4s and their regulation by proteins remains challenging due to the coexistence of multiple structures in a heterogeneous sample. Here, in this mini-review, we introduce the application of single-molecule force–spectroscopy methods, such as magnetic tweezers, optical tweezers, and atomic force microscopy, to characterize the polymorphism and folding/unfolding dynamics of G4s. We also briefly introduce recent studies using single-molecule force spectroscopy to study the molecular mechanisms of G4-interacting proteins.

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Submolecular dissection reveals strong and specific binding of polyamide–pyridostatin conjugates to human telomere interface

Cited by 20 publications

References 59 publications

Dissection of nanoconfinement and proximity effects on the binding events in DNA origami nanocavity

Dissection of nanoconfinement and proximity effects on the binding events in DNA origami nanocavity

Mechanical Stability of DNA Corona Phase on Gold Nanospheres

Characterization of G-Quadruplexes Folding/Unfolding Dynamics and Interactions with Proteins from Single-Molecule Force Spectroscopy

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