| Literature DB >> 31158262 |
Oren Kobiler1, Matthew D Weitzman2,3.
Abstract
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Year: 2019 PMID: 31158262 PMCID: PMC6546242 DOI: 10.1371/journal.ppat.1007714
Source DB: PubMed Journal: PLoS Pathog ISSN: 1553-7366 Impact factor: 6.823
Fig 1The cascade of events leading to RC formation.
Schematic illustration of viral genomes entering the nucleus and forming RCs. Viral genome (red line) is released from the capsid at the nuclear pore complex. Once inside the nucleus, transcription from IG of IE genes (viral mRNAs presented as orange lines) is initiated by the VP16 complex (yellow and gray structure). Viral transcripts are exported to the cytoplasm for translation of IE (purple circles), E (orange circles), and L (yellow circles) proteins by host ribosomes. In the nucleus, IE proteins induce GE and E gene expression. E proteins establish viral DNA replication and L gene expression in RCs (RC shown as orange area in the nucleus). E, early; GE, genome expansion; IE, immediate early; IG, incoming genome; L, late; RC, replication compartment; VP16, viral protein 16.
Fig 2Heterogeneity and interactions among RCs.
(A) Schematic illustration of an infected cell with two types of viral genomes (red or green lines) that form distinct RCs (RCs shown as orange area in the nucleus). Viral proteins within the RCs originate from the two genomes. Recombination events occur between two genomes in coalescing RCs (orange line). An entering genome that did not initiate an RC is also shown (condensed without background). (B, C) Fluorescence in situ hybridization image of U2OS (B) or Vero (C) cells 6 hours postinfection with two HSV-1 recombinants at MOI 20. Each viral recombinant carries a unique tag sequence that can be detected by a set of fluorescent probes (either green or red). Arrowhead points to a site of colocalization (indicating a possible recombination event). DNA staining was done by DAPI (gray). Scale bar, 20 μM. Experimental details were described [7]. MOI, multiplicity of infection; RC, replication compartment.