Erce MA, et al. (2013)

Reference: Erce MA, et al. (2013) Interactions affected by arginine methylation in the yeast protein-protein interaction network. Mol Cell Proteomics 12(11):3184-98

Reference Help

Abstract

Protein-protein interactions can be modulated by the methylation of arginine residues. As a means of testing this, we recently described a conditional two-hybrid system, based on the bacterial adenylate cyclase (BACTH) system. Here, we have used this conditional two-hybrid system to explore the effect of arginine methylation in modulating protein-protein interactions in a subset of the Saccharomyces cerevisiae arginine methylproteome network. Interactions between the yeast hub protein Npl3 and yeast proteins Air2, Ded1, Gbp2, Snp1, and Yra1 were first validated in the absence of methylation. The major yeast arginine methyltransferase Hmt1 was subsequently included in the conditional two-hybrid assay, initially to determine the degree of methylation that occurs. Proteins Snp1 and Yra1 were confirmed as Hmt1 substrates, with five and two novel arginine methylation sites mapped by ETD LC-MS/MS on these proteins, respectively. Proteins Ded1 and Gbp2, previously predicted but not confirmed as substrates of Hmt1, were also found to be methylated with five and seven sites mapped respectively. Air2 was found to be a novel substrate of Hmt1 with two sites mapped. Finally, we investigated the interactions of Npl3 with the five interaction partners in the presence of active Hmt1 and in the presence of Hmt1 with a G68R inactivation mutation. We found that the interaction between Npl3 and Air2, and Npl3 and Ded1, were significantly increased in the presence of active Hmt1; the interaction of Npl3 and Snp1 showed a similar degree of increase in interaction but this was not statistically significant. The interactions of Npl3 and Gbp2, along with Npl3 and Yra1, were not significantly increased or decreased by methylation. We conclude that methylarginine may be a widespread means by which the interactions of proteins are modulated.

Download Citation (.nbib)

Reference Type: Journal Article | Research Support, Non-U.S. Gov't
Authors: Erce MA, Abeygunawardena D, Low JK, Hart-Smith G, Wilkins MR
Primary Lit For
Additional Lit For
Review For

Gene Ontology Annotations

Evidence ID	Analyze ID	Gene/Complex	Systematic Name/Complex Accession	Qualifier	Gene Ontology Term ID	Gene Ontology Term	Aspect	Annotation Extension	Evidence	Method	Source	Assigned On	Reference

Download (.txt)

Analyze

Phenotype Annotations

Evidence ID	Analyze ID	Gene	Gene Systematic Name	Phenotype	Experiment Type	Experiment Type Category	Mutant Information	Strain Background	Chemical	Details	Reference

Download (.txt)

Analyze

Disease Annotations

Evidence ID	Analyze ID	Gene	Gene Systematic Name	Disease Ontology Term	Disease Ontology Term ID	Qualifier	Evidence	Method	Source	Assigned On		Reference

Download (.txt)

Analyze

Regulation Annotations

Evidence ID	Analyze ID	Regulator	Regulator Systematic Name	Target	Target Systematic Name	Direction	Regulation of	Happens During	Regulator Type	Direction	Regulation Of	Happens During	Method	Evidence	Strain Background	Reference

Download (.txt)

Analyze

Post-translational Modifications

				Site		Modification	Modifier	Source	Reference

Download (.txt)

Analyze

Interaction Annotations

Genetic Interactions

Evidence ID	Analyze ID		Interactor	Interactor Systematic Name	Interactor	Interactor Systematic Name	Allele	Assay	Annotation	Action	Phenotype	SGA score	P-value	Source	Reference	Note

Download (.txt)

Analyze

Physical Interactions

Evidence ID	Analyze ID		Interactor	Interactor Systematic Name	Interactor	Interactor Systematic Name	Assay	Annotation	Action	Modification	Source	Reference	Note

Download (.txt)

Analyze

Functional Complementation Annotations

Complement ID	Locus ID	Gene	Species	Gene ID	Strain background	Direction	Details	Source	Reference

Download (.txt)

Analyze

Published Datasets

Evidence ID	Analyze ID		Dataset	Description	Keywords	Number of Conditions	Reference

Download (.txt)

Analyze