The D10 Decapping Enzyme of Vaccinia Virus Contributes to Decay of Cellular and Viral mRNAs and to Virulence in Mice

Dunlap

Clinical Lymphoma Myeloma and Leukemia

2016

Introduction Multiple myeloma is a clonal malignancy of plasma B cells. While recent advances have improved overall prognosis, virtually all myeloma patients still succumb to relapsing disease. Therefore, novel therapies to treat this disease remain urgently needed. We have recently demonstrated that treatment of human multiple myeloma cells with an oncolytic virus known as myxoma results in rapid cell death even in the absence of viral replication; however, the specific mechanisms and pathways involved remain unknown. Materials and Methods To determine how Myxoma virus eliminates human multiple myeloma cells, we queried the apoptotic pathways which were activated following viral infection using immunoblot and other cell biology approaches. Results Our results indicate that myxoma virus infection initiates apoptosis in multiple myeloma cells through activation of the extrinsic initiator caspase-8. Caspase-8 activation subsequently results in cleavage of Bid and loss of mitochondrial membrane potential causing secondary activation of caspase-9. Activation of caspase-8 appears to be independent of extrinsic death ligands and instead correlates with depletion of cellular inhibitors of apoptosis. We hypothesize that this depletion results from virally mediated host-protein shutoff since a myxoma construct which overexpresses the viral decapping enzymes displays improved oncolytic potential. Conclusion Taken together, these results suggest that myxoma virus eliminates human multiple myeloma cells through a pathway unique to oncolytic poxviruses making it an excellent therapeutic option for the treatment of relapsed or refractory patients.

Section: Resultsmentioning

confidence: 99%

Myxoma Virus Induces Ligand Independent Extrinsic Apoptosis in Human Myeloma Cells

Dunlap

Clinical Lymphoma Myeloma and Leukemia

2016

Journal of General Virology

“…However, five conserved genes (G6R, I5L, F16L, D10R and A14.5L) have been defined as non-essential because single-gene-deletion mutants were created successfully (Betakova et al, 2000;Parrish & Moss, 2006;Senkevich et al, 2008;Sood et al, 2008;Senkevich et al, 2011;Liu et al, 2014). Four of these genes are known to affect virulence after infection of mice, suggesting that these genes were conserved because they carry out a crucial role in vivo (Betakova et al, 2000;Senkevich et al, 2008;Sood et al, 2008;Liu et al, 2014 (Meng et al, 2009). Other functions such as inhibition of apoptosis are redundant to some degree as well, with a hierarchy of importance across viral genes .…”

Section: Essential Genes As Defined By Single-genedeletion Mutantsmentioning

confidence: 99%

Redundancy complicates the definition of essential genes for vaccinia virus

Dobson

Tscharke

2015

Vaccinia virus (VACV) genes are characterized as either essential or non-essential for growth in culture. It seems intuitively obvious that if a gene can be deleted without imparting a growth defect in vitro it does not have a function related to basic replication or spread. However, this interpretation relies on the untested assumption that there is no redundancy across the genes that have roles in growth in cell culture. First, we provide a comprehensive summary of the literature that describes the essential genes of VACV. Next, we looked for interactions between large blocks of non-essential genes located at the ends of the genome by investigating sets of VACVs with large deletions at the genomic termini. Viruses with deletions at either end of the genome behaved as expected, exhibiting only mild or host-range defects. In contrast, combining deletions at both ends of the genome for the VACV Western Reserve (WR) strain caused a devastating growth defect on all cell lines tested. Unexpectedly, we found that the well-studied VACV growth factor homologue encoded by C11R has a role in growth in vitro that is exposed when 42 genes are absent from the left end of the VACV WR genome. These results demonstrate that some non-essential genes contribute to basic viral growth, but redundancy means these functions are not revealed by single-gene-deletion mutants.

“…The second category included genes associated with pre-mRNA splicing and maturation (DHX15, HNRNPF – two variants) and an mRNA de-capping enzyme, DCPS. Of note, viruses that carry their own de-capping enzymes, such as influenza and vaccinia viruses, use them to facilitate virus gene expression while inhibiting host translation (37, 38). Consequently, PA-X’s ability to up-regulate a host de-capping enzyme may provide an additional method for IAV to inhibit host translation.…”

Section: Discussionmentioning

confidence: 99%

Comparing the functions of equine and canine influenza H3N8 virus PA-X proteins: Suppression of reporter gene expression and modulation of global host gene expression

et al. 2016

The influenza PA-X protein is translated from the PA open reading frame from frameshifting and suppresses cellular gene expression due to its ribonuclease activity. We further defined the functional roles of PA-X by comparing PA-X proteins from two related viruses – equine influenza (EIV) and canine influenza (CIV) H3N8 – that differ in a C-terminal truncation and internal mutations. In vitro reporter gene assays revealed that both proteins were able to suppress gene expression. Interestingly, EIV PA-X demonstrated ~50% greater activity compared to CIV PA-X, and we identified the mutations that caused this difference. We used RNA-seq to evaluate the effects of PA-X on host gene expression after transfection into cultured cells. There were no significant differences in this property between EIV and CIV PA-X proteins, but expression of either resulted in the up-regulation of genes when compared to controls, most notably immunity-related proteins, trafficking proteins, and transcription factors.