Literature DB >> 22840425

JC virus agnoprotein enhances large T antigen binding to the origin of viral DNA replication: evidence for its involvement in viral DNA replication.

A Sami Saribas1, Martyn K White, Mahmut Safak.   

Abstract

Agnoprotein is required for the successful completion of the JC virus (JCV) life cycle and was previously shown to interact with JCV large T-antigen (LT-Ag). Here, we further characterized agnoprotein's involvement in viral DNA replication. Agnoprotein enhances the DNA binding activity of LT-Ag to the viral origin (Ori) without directly interacting with DNA. The predicted amphipathic α-helix of agnoprotein plays a major role in this enhancement. All three phenylalanine (Phe) residues of agnoprotein localize to this α-helix and Phe residues in general are known to play critical roles in protein-protein interaction, protein folding and stability. The functional relevance of all Phe residues was investigated by mutagenesis. When all were mutated to alanine (Ala), the mutant virus (F31AF35AF39A) replicated significantly less efficiently than each individual Phe mutant virus alone, indicating the importance of Phe residues for agnoprotein function. Collectively, these studies indicate a close involvement of agnoprotein in viral DNA replication.
Copyright © 2012 Elsevier Inc. All rights reserved.

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Year:  2012        PMID: 22840425      PMCID: PMC3444665          DOI: 10.1016/j.virol.2012.06.017

Source DB:  PubMed          Journal:  Virology        ISSN: 0042-6822            Impact factor:   3.616


  83 in total

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8.  The human polyoma JC virus agnoprotein acts as a viroporin.

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  22 in total

1.  A comprehensive proteomics analysis of JC virus Agnoprotein-interacting proteins: Agnoprotein primarily targets the host proteins with coiled-coil motifs.

Authors:  A Sami Saribas; Prasun K Datta; Mahmut Safak
Journal:  Virology       Date:  2019-10-20       Impact factor: 3.616

2.  The agnoprotein of polyomavirus JC is released by infected cells: evidence for its cellular uptake by uninfected neighboring cells.

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3.  Analysis of JC virus DNA replication using a quantitative and high-throughput assay.

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Review 4.  Expression of novel proteins by polyomaviruses and recent advances in the structural and functional features of agnoprotein of JC virus, BK virus, and simian virus 40.

Authors:  A Sami Saribas; Pascale Coric; Serge Bouaziz; Mahmut Safak
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5.  JC virus nucleotides 376-396 are critical for VP1 capsid protein expression.

Authors:  Laura C Ellis; Igor J Koralnik
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6.  Human polyoma JC virus minor capsid proteins, VP2 and VP3, enhance large T antigen binding to the origin of viral DNA replication: evidence for their involvement in regulation of the viral DNA replication.

Authors:  A Sami Saribas; Sarah Mun; Jaslyn Johnson; Mohammad El-Hajmoussa; Martyn K White; Mahmut Safak
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7.  Discovery and characterization of novel trans-spliced products of human polyoma JC virus late transcripts from PML patients.

Authors:  A Sami Saribas; Julia DeVoto; Akhil Golla; Hassen S Wollebo; Martyn K White; Mahmut Safak
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8.  Nuclear magnetic resonance structure revealed that the human polyomavirus JC virus agnoprotein contains an α-helix encompassing the Leu/Ile/Phe-rich domain.

Authors:  Pascale Coric; A Sami Saribas; Magid Abou-Gharbia; Wayne Childers; Martyn K White; Serge Bouaziz; Mahmut Safak
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9.  Nuclear Magnetic Resonance Structure of the Human Polyoma JC Virus Agnoprotein.

Authors:  Pascale Coric; A Sami Saribas; Magid Abou-Gharbia; Wayne Childers; Jon H Condra; Martyn K White; Mahmut Safak; Serge Bouaziz
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10.  Structure-based release analysis of the JC virus agnoprotein regions: A role for the hydrophilic surface of the major alpha helix domain in release.

Authors:  A Sami Saribas; Martyn K White; Mahmut Safak
Journal:  J Cell Physiol       Date:  2017-08-28       Impact factor: 6.384

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