Different Subcellular Localization of Theiler's Murine Encephalomyelitis Virus Leader Proteins of GDVII and DA Strains in BHK-21 Cells

Taniura, Naoko; Saito, Mineki; Okuwa, Takako; Saito, Ko; Ohara, Yoshikazu

doi:10.1128/jvi.02385-08

Cited by 7 publications

(11 citation statements)

References 31 publications

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“…On the other hand, the insertion of a 6-nt motif is an rare event in NDV evolution in view of the extremely low probability of nucleotide addition or deletion in the genome RNA of Paramyxoviruses [37,38]. Thus, it was most possible that genotype IX NDV was the common origin of genotype V-VIII.…”

Section: Discussionmentioning

confidence: 99%

Entire genome sequence analysis of genotype IX Newcastle disease viruses reveals their early-genotype phylogenetic position and recent-genotype genome size

Qiu

Sun

et al. 2011

Virol J

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BackgroundSix nucleotide (nt) insertion in the 5'-noncoding region (NCR) of the nucleoprotein (NP) gene of Newcaslte disease virus (NDV) is considered to be a genetic marker for recent genotypes of NDV, which emerged after 1960. However, F48-like NDVs from China, identified a 6-nt insert in the NP gene, have been previously classified into genotype III or genotype IX.ResultsIn order to clarify their phylogenetic position and explore the origin of NDVs with the 6-nt insert and its significance in NDV evolution, we determined the entire genome sequences of five F48-like viruses isolated in China between 1946 and 2002 by RT-PCR amplification of overlapping fragments of full-length genome and rapid amplification of cDNA ends. All the five NDV isolates shared the same genome size of 15,192-nt with the recent genotype V-VIII viruses whereas they had the highest homology with early genotype III and IV isolates.ConclusionsThe unique characteristic of the genome size and phylogenetic position of F48-like viruses warrants placing them in a separate geno-group, genotype IX. Results in this study also suggest that genotype IX viruses most likely originate from a genotype III virus by insertion of a 6-nt motif in the 5'-NCR of the NP gene which had occurred as early as in 1940 s, and might be the common origin of genotype V-VIII viruses.

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Section: Discussionmentioning

confidence: 99%

Entire genome sequence analysis of genotype IX Newcastle disease viruses reveals their early-genotype phylogenetic position and recent-genotype genome size

Qiu

Sun

et al. 2011

Virol J

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“…The L T -dependent apoptotic phenotypes (2), and L T intracellular localization differences (17) previously assigned to the S 57 (DA) and P 57 (GDVII) sequences, are now logically explained by the phosphorylation status of this residue. We do not yet know if GDVII or other viruses of this subtype use an alternative primary site instead.…”

Section: Resultsmentioning

confidence: 98%

“…Such viruses are also unable to inhibit stress granule formation (8). Equivalent mutations to the L T Ser/Thr domain (S 51 A, S 53 A, S 54 A) do not have similar effects (14), although a single amino acid change in the L T of GDVII virus (P 57 ) and DA virus (S 57 ) correlates with differential apoptotic phenotypes (2), and L T intracellular localization differences (17). …”

Section: Introductionmentioning

confidence: 99%

“…L T and L S also become phosphorylated, but at different sites than L E , and in reactions that do not require CK2 (15). Sequence comparisons have suggested S 57 (17) and/or T 63 (14) as possible sites in L T (DA). We now have experimental validation that L T (BeAn) and L S (SafV-2) and are differentially phosphorylated at S 57 (Ser/Thr domain) and T 58 (Theilo domain), respectively.…”

Section: Introductionmentioning

confidence: 99%

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AMP-activated protein kinase phosphorylates EMCV, TMEV and SafV leader proteins at different sites

Basta

Palmenberg

2014

Virology

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Cardioviruses of the Encephalomyocarditis virus (EMCV) and Theilovirus species, encode small, amino-terminal proteins called Leaders (L). Phosphorylation of the EMCV L (LE) at two distinct sites by CK2 and Syk kinases is important for virus-induced Nup phosphorylation and nucleocytoplasmic trafficking inhibition. Despite similar biological activities, the LE phosphorylation sites are not conserved in the Theiloviruses, Saffold virus (LS, SafV) or Theiler’s murine encephalitis virus (LT, TMEV) sequences even though these proteins also become phosphorylated in cells and cell-free extracts. Site prediction algorithms, combined with panels of site-specific protein mutations now identify analogous, but not homologous phosphorylation sites in the Ser/Thr and Theilo protein domains of LT and LS, respectively. In both cases, recombinant AMP-activated kinase (AMPK) was reactive with the proteins at these sites, and also with LE, modifying the same residue recognized by CK2.

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“…12 Moreover, the L protein of TMEV was reported to localize either 1 in both the nucleus and cytoplasm (DA strain) or 2 the cytoplasm only (GDVII strain). 13 The L protein of DA strain was known to interfere with the nucleocytoplasmic trafficking of cellular proteins; it promotes the redistribution of a nuclear protein to the cytoplasm and a cytoplasmic protein to the nucleus. 14 It was also demonstrated to inhibit the production of immediate-early alpha/beta interferon at the transcription level, 15 which led to the dysregulation of the whole cellular defense system by probably fostering the persistence of TMEV DA strain.…”

Section: Introductionmentioning

confidence: 99%

Intracellular localization of Saffold virus Leader (L) protein differs in Vero and HEp-2 cells

Victorio

et al. 2016

Emerging Microbes & Infections

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The Saffold virus (SAFV) genome is translated as a single long polyprotein precursor and co-translationally cleaved to yield 12 separate viral proteins. Little is known about the activities of SAFV proteins although their homologs in other picornaviruses have already been described. To further support research on functions and activities of respective viral proteins, we investigated the spatio-temporal distribution of SAFV proteins in Vero and HEp-2 cells that had been either transfected with plasmids that express individual viral proteins or infected with live SAFV. Our results revealed that, with the exception of the Leader (L) protein, all viral proteins were localized in the cytoplasm at all the time points assayed. The L protein was found in the cytoplasm at an early time point but was subsequently translocated to the nucleus of HEp-2, but not Vero, cells. This was observed in both transfected and infected cells. Further mutational analysis of L protein revealed that Threonine 58 of the Ser/Thr-rich domain of L protein is crucial for protein trafficking between the cytoplasm and nucleus in HEp-2 cells. These findings contribute to a deeper understanding and stimulate investigation of the differetial cellular responses of HEp-2 cells in comparison to other mammalian cell lines during SAFV infection.

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Different Subcellular Localization of Theiler's Murine Encephalomyelitis Virus Leader Proteins of GDVII and DA Strains in BHK-21 Cells

Cited by 7 publications

References 31 publications

Entire genome sequence analysis of genotype IX Newcastle disease viruses reveals their early-genotype phylogenetic position and recent-genotype genome size

Entire genome sequence analysis of genotype IX Newcastle disease viruses reveals their early-genotype phylogenetic position and recent-genotype genome size

AMP-activated protein kinase phosphorylates EMCV, TMEV and SafV leader proteins at different sites

Intracellular localization of Saffold virus Leader (L) protein differs in Vero and HEp-2 cells

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