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Development of a micro-neutralization assay for ebolaviruses using a replication-competent vesicular stomatitis hybrid virus and a quantitative PCR readout.

Vaccine.. 2017-10; 
Lee SS,Phy K,Peden K,Sheng-Fowler L.
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PCR Cloning and Subcloning ... The following glycoprotein genes were optimized for expression in human and African green monkey cells and synthesized (GenScript); each gene contained a 5′ NotI site and a 3′ PacI site for directional cloning into pVSV.4510. … Get A Quote

Abstract

Development of vaccines against highly pathogenic viruses that could also be used as agents of bioterrorism is both a public health issue and a national security priority. Methods that can quantify neutralizing antibodies will likely be crucial in demonstrating vaccine effectiveness, as most licensed viral vaccines are effective due to their capacity to elicit neutralizing antibodies. Assays to determine whether antibodies are neutralizing traditionally involve infectious virus, and the assay most commonly used is the plaque-reduction neutralization test (PRNT). However, when the virus is highly pathogenic, this assay must be done under the appropriate level of containment; for tier one select agents, such as E... More

Keywords

Ebolaviruses; Neutralization assay; RT-qPCR; VSV