Literature DB >> 15893559

Analysis of Ebola virus and VLP release using an immunocapture assay.

George Kallstrom1, Kelly L Warfield, Dana L Swenson, Shannon Mort, Rekha G Panchal, Gordon Ruthel, Sina Bavari, M Javad Aman.   

Abstract

Ebola virus (EBOV), an emerging pathogen, is the causative agent of a rapidly progressive hemorrhagic fever with high mortality rates. There are currently no approved vaccines or treatments available for Ebola hemorrhagic fever. Standard plaque assays are currently the only reliable techniques for enumerating the virus. Effective drug-discovery screening as well as target identification and validation require simple and more rapid detection methods. This report describes the development of a rapid ELISA that measures virus release with high sensitivity. This assay detects both Ebola virus and EBOV-like particles (VLPs) directly from cell-culture supernatants with the VP40 matrix protein serving as antigen. Using this assay, the contribution of the EBOV nucleocapsid (NC) proteins in VLP release was determined. These findings indicate that a combination of NC proteins together with the envelope components is optimal for VLP formation and release, a finding that is important for vaccination with Ebola VLPs. Furthermore, this assay can be used in surrogate models in non-biocontainment environment, facilitating both basic research on the mechanism of EBOV assembly and budding as well as drug-discovery research.

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Year:  2005        PMID: 15893559     DOI: 10.1016/j.jviromet.2005.02.015

Source DB:  PubMed          Journal:  J Virol Methods        ISSN: 0166-0934            Impact factor:   2.014


  24 in total

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9.  Zaire Ebola virus entry into human dendritic cells is insensitive to cathepsin L inhibition.

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10.  Ebolavirus is internalized into host cells via macropinocytosis in a viral glycoprotein-dependent manner.

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