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Richard W. Hardy

Researcher at Indiana University

Publications -  48
Citations -  2944

Richard W. Hardy is an academic researcher from Indiana University. The author has contributed to research in topics: RNA & Viral replication. The author has an hindex of 28, co-authored 46 publications receiving 2588 citations. Previous affiliations of Richard W. Hardy include University of Alabama at Birmingham & Washington University in St. Louis.

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Insect antiviral innate immunity: pathways, effectors, and connections.

TL;DR: An overview of the current understanding of the main insect antiviral pathways is provided and recent findings that further understand the roles of these pathways in facilitating a systemic and specific response to infecting viruses are examined.
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A Novel System for the Launch of Alphavirus RNA Synthesis Reveals a Role for the Imd Pathway in Arthropod Antiviral Response

TL;DR: Findings show that the Imd pathway mediates an antiviral response to Sindbis virus replication, the first demonstration of an anti-viral role for the ImD pathway in insects.
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Alphavirus RNA synthesis and non-structural protein functions.

TL;DR: This review describes what is currently understood about the regulation of alphavirus RNA synthesis, the roles of the viral non-structural proteins in this process and the functions of cis-acting RNA elements in replication, and points to open questions within the field.
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The Product of the Respiratory Syncytial Virus M2 Gene ORF1 Enhances Readthrough of Intergenic Junctions during Viral Transcription

TL;DR: Data show that the M2 protein functions as a transcriptional antiterminator that enhances the ability of the viral RNA polymerase to read through intergenic junctions and inhibit viral RNA replication and mRNA transcription.
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Functional cDNA Clones of the Human Respiratory Syncytial (RS) Virus N, P, and L Proteins Support Replication of RS Virus Genomic RNA Analogs and Define Minimal trans-Acting Requirements for RNA Replication

TL;DR: A system for expression and recovery of replicable RS virus RNA entirely from cDNA clones is developed that has the advantages that expression occurs at a level sufficient to allow direct biochemical analysis of the products of RNA replication and that neither the use of reporter genes nor wild-type RS helper virus is required.