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Tytuł pozycji:

Single-Molecule Dwell-Time Analysis of Restriction Endonuclease-Mediated DNA Cleavage.

Tytuł:
Single-Molecule Dwell-Time Analysis of Restriction Endonuclease-Mediated DNA Cleavage.
Autorzy:
Etson CM; Department of Chemistry, Tufts University; Department of Physics, Wesleyan University; .
Todorov P; Department of Chemistry, Tufts University.
Shatery Nejad N; Department of Physics, Wesleyan University.
Shrestha N; Department of Physics, Wesleyan University.
Walt DR; Department of Chemistry, Tufts University; Wyss Institute at Harvard University.
Źródło:
Journal of visualized experiments : JoVE [J Vis Exp] 2021 Feb 07 (168). Date of Electronic Publication: 2021 Feb 07.
Typ publikacji:
Journal Article; Research Support, N.I.H., Extramural; Video-Audio Media
Język:
English
Imprint Name(s):
Original Publication: [Boston, Mass. : MYJoVE Corporation, 2006]-
MeSH Terms:
DNA Cleavage*
DNA Restriction Enzymes/*metabolism
Single Molecule Imaging/*methods
Biotinylation ; DNA/metabolism ; Data Analysis ; Deoxyribonucleases, Type II Site-Specific/metabolism ; Kinetics ; Microfluidics ; Quantum Dots/chemistry ; Substrate Specificity ; Surface Properties ; Time Factors
Grant Information:
K12 GM074869 United States GM NIGMS NIH HHS
Substance Nomenclature:
9007-49-2 (DNA)
EC 3.1.21.- (DNA Restriction Enzymes)
EC 3.1.21.4 (Deoxyribonucleases, Type II Site-Specific)
Entry Date(s):
Date Created: 20210222 Date Completed: 20210319 Latest Revision: 20210319
Update Code:
20240105
DOI:
10.3791/62112
PMID:
33616095
Czasopismo naukowe
This novel total internal reflection fluorescence microscopy-based assay facilitates the simultaneous measurement of the length of the catalytic cycle for hundreds of individual restriction endonuclease (REase) molecules in one experiment. This assay does not require protein labeling and can be carried out with a single imaging channel. In addition, the results of multiple individual experiments can be pooled to generate well-populated dwell-time distributions. Analysis of the resulting dwell-time distributions can help elucidate the DNA cleavage mechanism by revealing the presence of kinetic steps that cannot be directly observed. Example data collected using this assay with the well-studied REase, EcoRV - a dimeric Type IIP restriction endonuclease that cleaves the palindromic sequence GAT↓ATC (where ↓ is the cut site) - are in agreement with prior studies. These results suggest that there are at least three steps in the pathway to DNA cleavage that is initiated by introducing magnesium after EcoRV binds DNA in its absence, with an average rate of 0.17 s -1 for each step.

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