2013
DOI: 10.1128/jvi.00321-13
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The Cellular Interactome of the Coronavirus Infectious Bronchitis Virus Nucleocapsid Protein and Functional Implications for Virus Biology

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Cited by 89 publications
(124 citation statements)
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References 79 publications
(91 reference statements)
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“…ACCEPTED MANUSCRIPT 16 Similarly, MKT-077 treatment also caused the reduction of NSP12-GFP, and the protein level was recoverable with the presence of proteasome inhibitor (Figure. 7).…”
Section: Accepted Manuscriptmentioning
confidence: 85%
See 1 more Smart Citation
“…ACCEPTED MANUSCRIPT 16 Similarly, MKT-077 treatment also caused the reduction of NSP12-GFP, and the protein level was recoverable with the presence of proteasome inhibitor (Figure. 7).…”
Section: Accepted Manuscriptmentioning
confidence: 85%
“…The interactome of PRRSV NSP12 was determined by high-affinity GFP pull-down coupled with label free mass spectrometry-based approach, which we have used previously to study virus/host protein interactions [16][17][18][19]. Our data identified112 cellular proteins probably interacted with NSP12, and these proteins were mainly nucleic acid binding proteins or chaperones and were grouped into several distinct functional clusters.…”
Section: Ifn-mediated Antiviral Responses In Order To Gain Time For Vmentioning
confidence: 89%
“…In recent years, a high-throughput, quantitative proteomic SILAC-based technique has been applied to study interactomes between viral proteins and host cellular proteins [41]. Most of these studies investigated the interactions between the viral and cellular proteins by using the overexpression of a target viral protein fused with a tag, such as green fluorescent protein in combination with a SILAC-based LC-MS/MS approach, coupled with immunoprecipitation and tag-trap beads [32,42]. This approach allows us to distinguish between cellular proteins that specifically bind to the viral protein and background binding proteins.…”
Section: Discussionmentioning
confidence: 99%
“…This has advantages over the yeast two-hybrid approach in that cell localization and post-translational modifications are not perturbed, as well as advantages over traditional TAP-tagging in that it is a quantitative rather than qualitative approach allowing the user to readily distinguish non-specifically interacting proteins and contaminants, from host factors that bind specifically. Further, as a sample is typically analyzed whole, rather than as individual protein bands, proteins of interest are not masked by similarly migrating proteins on a gel, nor do they typically need to be present at sufficient levels to be visible after staining, leading to increased numbers of confidently identified proteins 4 .…”
Section: Introductionmentioning
confidence: 99%
“…The results of this analysis are then processed to identify high confidence protein:protein interactions (Figure 1). SILAC immunoprecipitation enables the identification of not only direct interactions but also low affinity or indirect interactions with protein complexes 4 . Using this system, eIF4AI and II immunoprecipitations allowed reproducible and confident identification of the primary binding partner eIF4G (isoforms I/II and III)…”
Section: Introductionmentioning
confidence: 99%