Phosphorylation of Ser-80 of VP1 and Ser-254 of VP2 is essential for human BK virus propagation in tissue culture

Chen, Pei-Lain; Hsu, Pang-Hung; Fang, Chiung‐Yao; Chang, Chien‐Wen; Ou, Wei-Chih; Wang, Meilin; Chang, Deching

doi:10.1099/vir.0.033282-0

Cited by 6 publications

(7 citation statements)

References 51 publications

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“…Unfortunately, NCCR and full-genome sequencing shed little light on the origin of the contaminating virus, as BKPyV UT appears to be a relatively common variant, having been found in patient samples both in North Norway in 1990 (50) and in the United States in 2005 (51). Of note, this strain has also been used in several research labs (10,46,(72)(73)(74). Although we cannot pinpoint the infection temporally, we can be certain that BKPyV has been present in the cells at least since 2006 based on ATCC records.…”

Section: Discussionmentioning

confidence: 99%

The Human Fetal Glial Cell Line SVG p12 Contains Infectious BK Polyomavirus

Henriksen

Tylden

Dumoulin

et al. 2014

J Virol

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The human fetal glial cell line SVG was generated in 1985 by transfecting primary fetal brain cells with a plasmid containing an origin-defective mutant of simian virus 40 (SV40). The cells, which express SV40 large T-antigen, support the replication of human JC polyomavirus (JCPyV) and have been used for JCPyV studies but also for other studies in which cells of neural origin were desirable. We intended to use the SVG p12 cells from ATCC for antiviral drug studies with JCPyV. However, during initial experiments, immunofluorescence microscopy controls unexpectedly revealed cells expressing the late viral proteins VP1, VP2/ VP3, and agno. This was confirmed by Western blotting. Since our agnoprotein antiserum is specific for BKPyV agnoprotein, infection with BKPyV was suspected. Indeed, specific BKPyV PCR of SVG p12 supernatants revealed a viral load of >1 ؋ 10

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Section: Discussionmentioning

confidence: 99%

The Human Fetal Glial Cell Line SVG p12 Contains Infectious BK Polyomavirus

Henriksen

Tylden

Dumoulin

et al. 2014

J Virol

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“…Key VP1 residues for BKPyV assembly and entry have been identified by site directed mutagenesis [ 50 , 51 ]. Phosphorylation of Ser-80 of VP1 has been shown to be crucial for BKPyV propagation [ 52 ]. The receptor-binding site of BKPyV has been predicted to be located in a shallow groove formed by the BC and HI loops of VP1 [ 4 , 50 ].…”

Section: The Bkpyv Proteinsmentioning

confidence: 99%

“…In contrast, the mutation of the start codons of the minor capsid proteins alone or together reduced infectivity by over 99% compared to the WT demonstrating that these proteins are essential to create infectious virions [ 54 ]. Phosphorylation of Ser-254 of VP2 has been suggested to be critical for BKPyV propagation [ 52 ].…”

Section: The Bkpyv Proteinsmentioning

confidence: 99%

Biology of the BKPyV: An Update

Helle

Brochot

Handala

et al. 2017

Viruses

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The BK virus (BKPyV) is a member of the Polyomaviridae family first isolated in 1971. BKPyV causes frequent infections during childhood and establishes persistent infections with minimal clinical implications within renal tubular cells and the urothelium. However, reactivation of BKPyV in immunocompromised individuals may cause serious complications. In particular, with the implementation of more potent immunosuppressive drugs in the last decade, BKPyV has become an emerging pathogen in kidney and bone marrow transplant recipients where it often causes associated nephropathy and haemorrhagic cystitis, respectively. Unfortunately, no specific antiviral against BKPyV has been approved yet and the only therapeutic option is a modulation of the immunosuppressive drug regimen to improve immune control though it may increase the risk of rejection. A better understanding of the BKPyV life cycle is thus needed to develop efficient treatment against this virus. In this review, we provide an update on recent advances in understanding the biology of BKPyV.

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“…Previously, several PTMs were found in BKPyV structural proteins and minichromosomes [ 22 , 23 ]. The phosphorylation of BKPyV structural proteins is essential for viral propagation [ 24 ], but BKPyV LT protein modification has not been fully investigated. Phosphorylation of LT affects SV40 replication efficiency and interferes with host signaling pathways [ 25 , 26 ].…”

Section: Introductionmentioning

confidence: 99%

Histone deacetylase III interactions with BK polyomavirus large tumor antigen may affect protein stability

Hsu

Chao

Huang

et al. 2023

Virol J

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Background Human polyomavirus BK (BKPyV) causes associated nephropathy and contributes to urinary tract cancer development in renal transplant recipients. Large tumor antigen (LT) is an early protein essential in the polyomavirus life cycle. Protein acetylation plays a critical role in regulating protein stability, so this study investigated the acetylation of the BKPyV LT protein. Methods The BKPyV LT nucleotide was synthesized, and the protein was expressed by transfection into permissive cells. The BKPyV LT protein was immunoprecipitated and subjected to LC-MS/MS analysis to determine the acetylation residues. The relative lysine was then mutated to arginine in the LT nucleotide and BKPyV genome to analyze the role of LT lysine acetylation in the BKPyV life cycle. Results BKPyV LT acetylation sites were identified at Lys3 and Lys230 by mass spectrometry. HDAC3 and HDAC8 and their deacetylation activity are required for BKPyV LT expression. In addition, mutations of Lys3 and Lys230 to arginine increased LT expression, and the interaction of HDAC3 and LT was confirmed by coimmunoprecipitation. Conclusions HDAC3 is a newly identified protein that interacts with BKPyV LT, and LT acetylation plays a vital role in the BKPyV life cycle.

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Phosphorylation of Ser-80 of VP1 and Ser-254 of VP2 is essential for human BK virus propagation in tissue culture

Cited by 6 publications

References 51 publications

The Human Fetal Glial Cell Line SVG p12 Contains Infectious BK Polyomavirus

The Human Fetal Glial Cell Line SVG p12 Contains Infectious BK Polyomavirus

Biology of the BKPyV: An Update

Histone deacetylase III interactions with BK polyomavirus large tumor antigen may affect protein stability

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