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A recombinant transmissible gastroenteritis coronavirus (rTGEV) in which E gene was deleted (rTGEV-DeltaE) has been engineered. This deletion mutant only grows in cells expressing E protein (E(+) cells) indicating that E was an essential gene for TGEV replication. Electron microscopy studies of rTGEV-DeltaE infected BHK-pAPN-E(-) cells showed that only immature intracellular virions were assembled. These virions were non-infectious and not secreted to the extracellular medium in BHK-pAPN-E(-) cells. RNA and protein composition analysis by RNase-gold and immunoelectron microscopy showed that rTGEV-DeltaE virions contained RNA and also all the structural TGEV proteins, except the deleted E protein. Nevertheless, full virion maturation was blocked. Studies of the rTGEV-DeltaE subcellular localization by confocal and immunoelectron microscopy in infected E(-) cells showed that in the absence of E protein virus trafficking was arrested in the intermediate compartment. Therefore, the absence of E protein in TGEV resulted in two actions, a blockade of virus trafficking in the membranes of the secretory pathway, and prevention of full virus maturation.
E protein, Genes, Essential, Swine, Transmissible gastroenteritis virus, Virion, Virus Replication, Virus maturation, Article, Cell Line, Coronavirus, Viral Proteins, Viral Envelope Proteins, TGEV, Virology, Cricetinae, Animals, LLC-PK1 Cells, Nidovirus, Gene Deletion
E protein, Genes, Essential, Swine, Transmissible gastroenteritis virus, Virion, Virus Replication, Virus maturation, Article, Cell Line, Coronavirus, Viral Proteins, Viral Envelope Proteins, TGEV, Virology, Cricetinae, Animals, LLC-PK1 Cells, Nidovirus, Gene Deletion
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