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Structures of prM-containing dengue and yellow fever virus particles were determined to 16 and 25 A resolution, respectively, by cryoelectron microscopy and image reconstruction techniques. The closely similar structures show 60 icosahedrally organized trimeric spikes on the particle surface. Each spike consists of three prM:E heterodimers, where E is an envelope glycoprotein and prM is the precursor to the membrane protein M. The pre-peptide components of the prM proteins in each spike cover the fusion peptides at the distal ends of the E glycoproteins in a manner similar to the organization of the glycoproteins in the alphavirus spikes. Each heterodimer is associated with an E and a prM transmembrane density. These transmembrane densities represent either an EE or prMprM antiparallel coiled coil by which each protein spans the membrane twice, leaving the C-terminus of each protein on the exterior of the viral membrane, consistent with the predicted membrane-spanning domains of the unprocessed polyprotein.
Models, Molecular, 570, Flavivirus, Cryoelectron Microscopy, Lipid Bilayers, 610, Dengue Virus, Cell Line, Viral Proteins, Image Processing, Computer-Assisted, Animals, Sindbis Virus, Yellow fever virus, Nucleocapsid
Models, Molecular, 570, Flavivirus, Cryoelectron Microscopy, Lipid Bilayers, 610, Dengue Virus, Cell Line, Viral Proteins, Image Processing, Computer-Assisted, Animals, Sindbis Virus, Yellow fever virus, Nucleocapsid
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