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Dive into the research topics where Daniel L. Floyd is active.

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Featured researches published by Daniel L. Floyd.


Proceedings of the National Academy of Sciences of the United States of America | 2008

Single-particle kinetics of influenza virus membrane fusion.

Daniel L. Floyd; Justin R. Ragains; John J. Skehel; Stephen C. Harrison; Antoine M. van Oijen

Membrane fusion is an essential step during entry of enveloped viruses into cells. Conventional fusion assays are generally limited to observation of ensembles of multiple fusion events, confounding more detailed analysis of the sequence of the molecular steps involved. We have developed an in vitro, two-color fluorescence assay to monitor kinetics of single virus particles fusing with a target bilayer on an essentially fluid support. Analysis of lipid- and content-mixing trajectories on a particle-by-particle basis provides evidence for multiple, long-lived kinetic intermediates leading to hemifusion, followed by a single, rate-limiting step to pore formation. We interpret the series of intermediates preceding hemifusion as a result of the requirement that multiple copies of the trimeric hemagglutinin fusion protein be activated to initiate the fusion process.


Biophysical Journal | 2010

Analysis of Kinetic Intermediates in Single-Particle Dwell-Time Distributions

Daniel L. Floyd; Stephen C. Harrison; Antoine M. van Oijen

Many biological and chemical processes proceed through one or more intermediate steps. Statistical analysis of dwell-time distributions from single molecule trajectories enables the study of intermediate steps that are not directly observable. Here, we discuss the application of the randomness parameter and model fitting in determining the number of steps in a stochastic process. Through simulated examples, we show some of the limitations of these techniques. We discuss how shot noise and heterogeneity among the transition rates of individual steps affect how accurately the number of steps can be determined. Finally, we explore dynamic disorder in multistep reactions and show that the phenomenon can obscure the presence of rate-limiting intermediate steps.


Optics Express | 2013

Single particle detection in CMOS compatible photonic crystal nanobeam cavities

Qimin Quan; Daniel L. Floyd; Ian B. Burgess; Parag B. Deotare; Ian W. Frank; Sindy K. Y. Tang; Rob Ilic; Marko Loncar

We report the label-free detection of single particles using photonic crystal nanobeam cavities fabricated in silicon-on-insulator platform, and embedded inside microfluidic channels fabricated in poly-dimethylsiloxane (PDMS). Our system operates in the telecommunication wavelength band, thus leveraging the widely available, robust and tunable telecom laser sources. Using this approach, we demonstrated the detection of polystyrene nanoparticles with dimensions down to 12.5nm in radius. Furthermore, binding events of a single streptavidin molecule have been observed.


PLOS ONE | 2012

Kinetics of Proton Transport into Influenza Virions by the Viral M2 Channel

Tijana Ivanovic; Rutger Rozendaal; Daniel L. Floyd; Miloš A. Popović; Antoine M. van Oijen; Stephen C. Harrison

M2 protein of influenza A viruses is a tetrameric transmembrane proton channel, which has essential functions both early and late in the virus infectious cycle. Previous studies of proton transport by M2 have been limited to measurements outside the context of the virus particle. We have developed an in vitro fluorescence-based assay to monitor internal acidification of individual virions triggered to undergo membrane fusion. We show that rimantadine, an inhibitor of M2 proton conductance, blocks the acidification-dependent dissipation of fluorescence from a pH-sensitive virus-content probe. Fusion-pore formation usually follows internal acidification but does not require it. The rate of internal virion acidification increases with external proton concentration and saturates with a pKm of ∼4.7. The rate of proton transport through a single, fully protonated M2 channel is approximately 100 to 400 protons per second. The saturating proton-concentration dependence and the low rate of internal virion acidification derived from authentic virions support a transporter model for the mechanism of proton transfer.


Journal of Visualized Experiments | 2009

Method for Measurement of Viral Fusion Kinetics at the Single Particle Level

Daniel L. Floyd; Stephen C. Harrison; Antoine M. van Oijen

Membrane fusion is an essential step during entry of enveloped viruses into cells. Conventional fusion assays typically report on a large number of fusion events, making it difficult to quantitatively analyze the sequence of the molecular steps involved. We have developed an in vitro, two-color fluorescence assay to monitor kinetics of single virus particles fusing with a target bilayer on an essentially fluid support. Influenza viral particles are incubated with a green lipophilic fluorophore to stain the membrane and a red hydrophilic fluorophore to stain the viral interior. We deposit a ganglioside-containing lipid bilayer on the dextran-functionilized glass surface of a flow cell, incubate the viral particles on the planar bilayer and image the fluorescence of a 100 x 100 μm2 area, containing several hundreds of particles, on a CCD camera. By imaging both the red and green fluorescence, we can simultaneously monitor the behavior of the membrane dye (green) and the aqueous content (red) of the particles. Upon lowering the pH to a value below the fusion pH, the particles will fuse with the membrane. Hemifusion, the merging of the outer leaflet of the viral membrane with the outer leaflet of the target membrane, will be visible as a sudden change in the green fluorescence of a particle. Upon the subsequent fusion of the two remaining distal leaflets a pore will be formed and the red-emitting fluorophore in the viral particle will be released under the target membrane. This event will give rise to a decrease of the red fluorescence of individual particles. Finally, the integrated fluorescence from a pH-sensitive fluorophore that is embedded in the target membrane reports on the exact time of the pH drop. From the three fluorescence-time traces, all the important events (pH drop, lipid mixing upon hemifusion, content mixing upon pore formation) can now be extracted in a straightforward manner and for every particle individually. By collecting the elapsed times for the various transitions for many individual particles in histograms, we can determine the lifetimes of the corresponding intermediates. Even hidden intermediates that do not have a direct fluorescent observable can be visualized directly from these histograms.


conference on lasers and electro optics | 2012

High-Q, low index-contrast polymeric photonic crystal nanobeam cavities

Qimin Quan; Ian B. Burgess; Sindy K. Y. Tang; Daniel L. Floyd; Marko Loncar

We present the realization of high-Q (Q=36,000) polymeric photonic crystal nanobeam cavities made of two polymers that have an ultra-low index contrast (ratio=1.15), and demonstrate that these polymer cavities are outstanding refractive index sensors (FOM=9190).


Nanoscale | 2013

Size-controlled fluorescent nanodiamonds: a facile method of fabrication and color-center counting

Remi Mahfouz; Daniel L. Floyd; Wei Peng; Jennifer T. Choy; Marko Loncar; Osman M. Bakr


Archive | 2008

COMPOUNDS AND METHODS FOR ASSAYING FUSION OF AN INDIVIDUAL, ENVELOPED VIRUS WITH TARGET MEMBRANE

Antoine M. van Oijen; Daniel L. Floyd


15th International Conference on Miniaturized Systems for Chemistry and Life Sciences 2011, MicroTAS 2011 | 2011

LABEL-FREE SENSING WITH PHOTONIC CRYSTAL NANOBEAM CAVITIES

Qimin Quan; Ian B. Burgess; Sindy K. Y. Tang; Daniel L. Floyd; Parag B. Deotare; Ian W. Frank; Rob Ilic; Frank Vollmer; Marko Loncar


Biophysical Journal | 2010

Lipid Bilayer Rigidity Affects the Fusion Kinetics of Individually Observed Influenza Particles

Jason J. Otterstrom; Daniel L. Floyd; John J. Skehel; Stephen C. Harrison; Antoine M. van Oijen

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Stephen C. Harrison

Howard Hughes Medical Institute

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Parag B. Deotare

Massachusetts Institute of Technology

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