Single-particle kinetics of influenza virus membrane fusion

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

doi:10.1073/pnas.0807771105

Cited by 262 publications

(419 citation statements)

References 42 publications

(51 reference statements)

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“…Our data reveal a need for two to three HA trimers for fusion and strongly support a kinetic model of HA-mediated fusion requiring simultaneous action of multiple, neighboring trimers (15,16). This model requires only the stochastic behavior of the HA trimers in combination with a high HA surface density.…”

Section: Discussionmentioning

confidence: 56%

“…Fluorescence intensity from individual IgG/Fab molecules adsorbed to clean glass in pH 5.0 buffer was acquired under identical illumination conditions. Data analysis was performed using custom MATLAB (Mathworks, Inc.) scripts, similar to those previously described (15,29). Briefly, viruses were identified in the red channel and paired with separately identified locations in the green channel.…”

Section: Methodsmentioning

confidence: 99%

“…In this manner, we obtain information about the speed of the rate-limiting step along the fusion pathway and the number of rate-limiting steps. This latter value has been shown to represent the number of HA required for fusion (15). This kinetic analysis requires at least 50 events to have the statistical power to determine the number of HA trimers involved (39) and because increasing IgG/Fab concentrations results in fewer fusing virions, not all concentrations could be analyzed (SI Materials and Methods).…”

Section: Low Occupancies Can Significantly Reduce the Extent Of Hemifmentioning

confidence: 99%

“…Refolding of the protein brings the viral and endosomal membranes close together and catalyzes their fusion (11,12). Several biophysical studies indicate that multiple HA trimers must work together by coordinating their conformational changes for membrane fusion to occur (13)(14)(15)(16).…”

mentioning

confidence: 99%

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Relating influenza virus membrane fusion kinetics to stoichiometry of neutralizing antibodies at the single-particle level

Otterstrom

Brandenburg

Koldijk

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

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The ability of antibodies binding the influenza hemagglutinin (HA) protein to neutralize viral infectivity is of key importance in the design of next-generation vaccines and for prophylactic and therapeutic use. The two antibodies CR6261 and CR8020 have recently been shown to efficiently neutralize influenza A infection by binding to and inhibiting the influenza A HA protein that is responsible for membrane fusion in the early steps of viral infection. Here, we use single-particle fluorescence microscopy to correlate the number of antibodies or antibody fragments (Fab) bound to an individual virion with the capacity of the same virus particle to undergo membrane fusion. To this end, individual, infectious virus particles bound by fluorescently labeled antibodies/ Fab are visualized as they fuse to a planar, supported lipid bilayer. The fluorescence intensity arising from the virus-bound antibodies/ Fab is used to determine the number of molecules attached to viral HA while a fluorescent marker in the viral membrane is used to simultaneously obtain kinetic information on the fusion process. We experimentally determine that the stoichiometry required for fusion inhibition by both antibody and Fab leaves large numbers of unbound HA epitopes on the viral surface. Kinetic measurements of the fusion process reveal that those few particles capable of fusion at high antibody/Fab coverage display significantly slower hemifusion kinetics. Overall, our results support a membrane fusion mechanism requiring the stochastic, coordinated action of multiple HA trimers and a model of fusion inhibition by stem-binding antibodies through disruption of this coordinated action.influenza | neutralizing antibody | hemagglutinin | neutralization stoichiometry | membrane fusion

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Section: Discussionmentioning

confidence: 56%

Section: Methodsmentioning

confidence: 99%

Section: Low Occupancies Can Significantly Reduce the Extent Of Hemifmentioning

confidence: 99%

mentioning

confidence: 99%

See 2 more Smart Citations

Relating influenza virus membrane fusion kinetics to stoichiometry of neutralizing antibodies at the single-particle level

Otterstrom

Brandenburg

Koldijk

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

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“…This modification also resulted in SNAP25-dependent fusion 24 . Bilayers cushioned on a soft polymer layer had been known to better preserve transmembrane protein mobility and function 32 , and had been used in fusion studies with viruses 33 . In addition, PEGylated bilayers seem to retain some ability to self-heal and are very robust 34,35 .…”

Section: Introductionmentioning

confidence: 99%

SNARE-mediated Fusion of Single Proteoliposomes with Tethered Supported Bilayers in a Microfluidic Flow Cell Monitored by Polarized TIRF Microscopy

Nikolaus

Karatekin

2016

JoVE

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In the ubiquitous process of membrane fusion the opening of a fusion pore establishes the first connection between two formerly separate compartments. During neurotransmitter or hormone release via exocytosis, the fusion pore can transiently open and close repeatedly, regulating cargo release kinetics. Pore dynamics also determine the mode of vesicle recycling; irreversible resealing results in transient, "kiss-and-run" fusion, whereas dilation leads to full fusion. To better understand what factors govern pore dynamics, we developed an assay to monitor membrane fusion using polarized total internal reflection fluorescence (TIRF) microscopy with single molecule sensitivity and ~15 msec time resolution in a biochemically well-defined in vitro system. Fusion of fluorescently labeled small unilamellar vesicles containing v-SNARE proteins (v-SUVs) with a planar bilayer bearing t-SNAREs, supported on a soft polymer cushion (t-SBL, t-supported bilayer), is monitored. The assay uses microfluidic flow channels that ensure minimal sample consumption while supplying a constant density of SUVs. Exploiting the rapid signal enhancement upon transfer of lipid labels from the SUV to the SBL during fusion, kinetics of lipid dye transfer is monitored. The sensitivity of TIRF microscopy allows tracking single fluorescent lipid labels, from which lipid diffusivity and SUV size can be deduced for every fusion event. Lipid dye release times can be much longer than expected for unimpeded passage through permanently open pores. Using a model that assumes retardation of lipid release is due to pore flickering, a pore "openness", the fraction of time the pore remains open during fusion, can be estimated. A soluble marker can be encapsulated in the SUVs for simultaneous monitoring of lipid and soluble cargo release. Such measurements indicate some pores may reseal after losing a fraction of the soluble cargo. Video LinkThe video component of this article can be found at

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Protein–lipid interactions critical to replication of the influenza A virus

Chlanda

Zimmerberg

2016

FEBS Letters

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Influenza A virus (IAV) assembles on the plasma membrane where viral proteins localize to form a bud encompassing the viral genome, which ultimately pinches off to give rise to newly formed infectious virions. Upon entry, the virus faces the opposite task—fusion with the endosomal membrane and disassembly to deliver the viral genome to the cytoplasm. There are at least four influenza proteins—hemagglutinin (HA), neuraminidase (NA), matrix 1 protein (M1), and the M2 ion channel—that are known to directly interact with the cellular membrane and modify membrane curvature in order to both assemble and disassemble membrane-enveloped virions. Here, we summarize and discuss current knowledge of the interactions of lipids and membrane proteins involved in the IAV replication cycle.

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Single-particle kinetics of influenza virus membrane fusion

Cited by 262 publications

References 42 publications

Relating influenza virus membrane fusion kinetics to stoichiometry of neutralizing antibodies at the single-particle level

Relating influenza virus membrane fusion kinetics to stoichiometry of neutralizing antibodies at the single-particle level

SNARE-mediated Fusion of Single Proteoliposomes with Tethered Supported Bilayers in a Microfluidic Flow Cell Monitored by Polarized TIRF Microscopy

Protein–lipid interactions critical to replication of the influenza A virus

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