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Bryan R. Cullen

Researcher at Duke University

Publications -  376
Citations -  52946

Bryan R. Cullen is an academic researcher from Duke University. The author has contributed to research in topics: RNA & Gene. The author has an hindex of 121, co-authored 371 publications receiving 50901 citations. Previous affiliations of Bryan R. Cullen include Hoffmann-La Roche & University of Medicine and Dentistry of New Jersey.

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Mechanism of action of regulatory proteins encoded by complex retroviruses.

TL;DR: Data demonstrate that retrovirally encoded transcriptional trans-activators can exert a similar effect by several very different mechanisms, and posttranscriptional regulation of retroviral gene expression appears to occur via a single pathway that is probably dependent on the recruitment of a highly conserved cellular cofactor.
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A single amino acid difference in the host APOBEC3G protein controls the primate species specificity of HIV type 1 virion infectivity factor

TL;DR: It is demonstrated that a single APOBEC3G residue controls the ability of the HIV-1 Vif protein to bind and inactivate these host defense factors, suggesting the biological barrier preventing the entry of additional SIV into the human population as zoonotic infections is potentially quite fragile.
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Transcriptional interference in avian retroviruses--implications for the promoter insertion model of leukaemogenesis.

TL;DR: The downstream (3′) long terminal repeat of an avian retroviral provirus is unable to act as an efficient promoter of transcription when a transcriptionally active upstream (5′) LTR is present.
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Nuclear mRNA export: insights from virology.

TL;DR: Efforts to identify the cellular targets of these viral proteins and RNA elements have led to the identification of Crm1 and Tap as essential human nuclear RNA-export factors and continue to provide insights into how mRNAs are selected for export.
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Overexpression of Exportin 5 enhances RNA interference mediated by short hairpin RNAs and microRNAs

TL;DR: It is demonstrated that overexpressed sh RNAs can saturate the activity of endogenous Exportin 5, a factor required for nuclear export of both shRNAs and pre-miRNAs, and simultaneous overexpression of exportin 5 reverses this effect.