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CMP
Credit: Jack Hobhouse

Professor Achillefs Kapanidis

Professor of Biological Physics

Research theme

  • Biological physics

Sub department

  • Condensed Matter Physics

Research groups

  • Gene machines
Achillefs.Kapanidis@physics.ox.ac.uk
Telephone: 01865 (2)72226
Biochemistry Building
groups.physics.ox.ac.uk/genemachines/group
  • About
  • Publications

Retention of transcription initiation factor σ70 in transcription elongation: single-molecule analysis

Molecular Cell 20 (2005) 347-356

Authors:

A Kapanidis, Margeat E, Laurence TA, Doose S
More details from the publisher
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Alternating-Laser Excitation of Single Molecules

Accounts of Chemical Research American Chemical Society (ACS) 38:10 (2005) 824-824

Authors:

Achillefs N Kapanidis, Ted A Laurence, Nam Ki Lee, Emmanuel Margeat, Xiangxu Kong, Shimon Weiss
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Alternating‐Laser Excitation of Single Molecules

ChemInform Wiley 36:39 (2005) no-no

Authors:

Achillefs N Kapanidis, Ted A Laurence, Nam Ki Lee, Emmanuel Margeat, Xiangxu Kong, Shimon Weiss
More details from the publisher

Alternating-laser excitation of single molecules.

Acc Chem Res 38:7 (2005) 523-533

Authors:

Achillefs N Kapanidis, Ted A Laurence, Nam Ki Lee, Emmanuel Margeat, Xiangxu Kong, Shimon Weiss

Abstract:

Single-molecule fluorescence spectroscopy addresses biological mechanisms and enables ultrasensitive diagnostics. We describe a new family of single-molecule fluorescence methods that uses alternating-laser excitation (ALEX) of diffusing or immobilized biomolecules to study their structure, interactions, and dynamics. This is accomplished using ratios that report on the distance between and the stoichiometry of fluorophores attached to the molecules of interest. The principle of alternation is compatible with several time scales, allowing monitoring of fast dynamics or simultaneous monitoring of a large number of individual molecules.
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Accurate FRET measurements within single diffusing biomolecules using alternating-laser excitation.

Biophys J 88:4 (2005) 2939-2953

Authors:

Nam Ki Lee, Achillefs N Kapanidis, You Wang, Xavier Michalet, Jayanta Mukhopadhyay, Richard H Ebright, Shimon Weiss

Abstract:

Fluorescence resonance energy transfer (FRET) between a donor (D) and an acceptor (A) at the single-molecule level currently provides qualitative information about distance, and quantitative information about kinetics of distance changes. Here, we used the sorting ability of confocal microscopy equipped with alternating-laser excitation (ALEX) to measure accurate FRET efficiencies and distances from single molecules, using corrections that account for cross-talk terms that contaminate the FRET-induced signal, and for differences in the detection efficiency and quantum yield of the probes. ALEX yields accurate FRET independent of instrumental factors, such as excitation intensity or detector alignment. Using DNA fragments, we showed that ALEX-based distances agree well with predictions from a cylindrical model of DNA; ALEX-based distances fit better to theory than distances obtained at the ensemble level. Distance measurements within transcription complexes agreed well with ensemble-FRET measurements, and with structural models based on ensemble-FRET and x-ray crystallography. ALEX can benefit structural analysis of biomolecules, especially when such molecules are inaccessible to conventional structural methods due to heterogeneity or transient nature.
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