PRISMA: Protein Interaction Screen on Peptide Matrix Reveals Interaction Footprints and Modifications- Dependent Interactome of Intrinsically Disordered C/EBPβ

Dittmar, Gunnar; Hernández, Daniel; Kowenz‐Leutz, Elisabeth; Kirchner, Marieluise; Kahlert, Günther; Wesołowski, Radosław; Baum, Katharina; Knoblich, Maria; Hofstätter, Maria; Muller, Arnaud; Wolf, Jana; Reimer, Ulf; Leutz, Achim

doi:10.1016/j.isci.2019.02.026

Cited by 35 publications

(70 citation statements)

References 74 publications

(105 reference statements)

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“…A screening technique targeting transient SLiM-based interactions along the primary structure was recently developed. The technique, PrISMa (Protein Interaction Screen on a Peptide Matrix), is based on a membrane-bound array of overlapping peptides, spanning the entire sequence of the protein of interest, creating a sliding window for the detection of SLiM-mediated interactions [ 11 ] (Fig. 1d, f ).…”

Section: Peptide Array–based Interaction Screensmentioning

confidence: 99%

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Peptide array–based interactomics

Hernández

Dittmar

2021

Anal Bioanal Chem

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The analysis of protein-protein interactions (PPIs) is essential for the understanding of cellular signaling. Besides probing PPIs with immunoprecipitation-based techniques, peptide pull-downs are an alternative tool specifically useful to study interactome changes induced by post-translational modifications. Peptides for pull-downs can be chemically synthesized and thus offer the possibility to include amino acid exchanges and post-translational modifications (PTMs) in the pull-down reaction. The combination of peptide pull-down and analysis of the binding partners with mass spectrometry offers the direct measurement of interactome changes induced by PTMs or by amino acid exchanges in the interaction site. The possibility of large-scale peptide synthesis on a membrane surface opened the possibility to systematically analyze interactome changes for mutations of many proteins at the same time. Short linear motifs (SLiMs) are amino acid patterns that can mediate protein binding. A significant number of SLiMs are located in regions of proteins, which are lacking a secondary structure, making the interaction motifs readily available for binding reactions. Peptides are particularly well suited to study protein interactions, which are based on SLiM-mediated binding. New technologies using arrayed peptides for interaction studies are able to identify SLIM-based interaction and identify the interaction motifs. Graphical abstract

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Section: Peptide Array–based Interaction Screensmentioning

confidence: 99%

“…1g ). The technique was used to map the interactome of the transcription factor C/EBPβ, identifying a large number of new interaction partners [ 11 ].…”

Section: Peptide Array–based Interaction Screensmentioning

confidence: 99%

Peptide array–based interactomics

Hernández

Dittmar

2021

Anal Bioanal Chem

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“…High Throughput Peptide-based Interaction Proteomics-Recently, the advantageous parts of both above-mentioned peptide pull-down approaches have been combined (Fig. 2): Instead of probing a peptide array with a single prey protein, peptide arrays were probed with whole cell lysates and interacting proteins were identified using quantitative mass spectrometry (28,29,40). In all three cases, 14 -18 mer peptides were synthesized on cellulose membranes via the SPOT technology that were then incubated with cell extracts to identify binding partners via mass spectrometry.…”

Section: Peptide-based Interaction Proteomicsmentioning

confidence: 99%

“…The two other studies therefore employed quantification to distinguish specific from nonspecific binders. Dittmar and co-workers used a sliding window approach (overlapping "tiled" peptides) to map binding partners along the sequence of C/EBPbeta (28). They also assessed the impact of PTMs because SPOT synthesis permits inclusion of phosphorylation, methylation (mono, di, tri), citrullination, acetylation, crotonylation, sumoylation and many more.…”

Section: Peptide-based Interaction Proteomicsmentioning

confidence: 99%

“…For the actual pull-down experiment, it is advantageous to use a cell extract that contains the putative interaction partners. For example, for interactions in the neuronal context it makes sense to use extract from neuronal cell lines (29), and for interaction partners of nuclear proteins nuclear extracts are a good choice (28). Whatever extract is used, it should be rather concentrated (5 mg protein/ml) to increase the sensitivity of the screen (28,29).…”

Section: Peptide-based Interaction Proteomicsmentioning

confidence: 99%

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Peptide-based Interaction Proteomics

Meyer

Selbach

2020

Molecular & Cellular Proteomics

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Protein-protein interactions are often mediated by short linear motifs (SLiMs) that are located in intrinsically disordered regions (IDRs) of proteins. Interactions mediated by SLiMs are notoriously difficult to study, and many functionally relevant interactions likely remain to be uncovered. Recently, pull-downs with synthetic peptides in combination with quantitative mass spectrometry emerged as a powerful screening approach to study protein-protein interactions mediated by SLiMs. Specifically, arrays of synthetic peptides immobilized on cellulose membranes provide a scalable means to identify the interaction partners of many peptides in parallel. In this minireview we briefly highlight the relevance of SLiMs for protein-protein interactions, outline existing screening technologies, discuss unique advantages of peptide-based interaction screens and provide practical suggestions for setting up such peptide-based screens.

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