Passa al contenuto
Merck

Global analysis of RNA-binding protein dynamics by comparative and enhanced RNA interactome capture.

Nature protocols (2020-11-20)
Joel I Perez-Perri, Marko Noerenberg, Wael Kamel, Caroline E Lenz, Shabaz Mohammed, Matthias W Hentze, Alfredo Castello
ABSTRACT

Interactions between RNA-binding proteins (RBPs) and RNAs are critical to cell biology. However, methods to comprehensively and quantitatively assess these interactions within cells were lacking. RNA interactome capture (RIC) uses in vivo UV crosslinking, oligo(dT) capture, and proteomics to identify RNA-binding proteomes. Recent advances have empowered RIC to quantify RBP responses to biological cues such as metabolic imbalance or virus infection. Enhanced RIC exploits the stronger binding of locked nucleic acid (LNA)-containing oligo(dT) probes to poly(A) tails to maximize RNA capture selectivity and efficiency, profoundly improving signal-to-noise ratios. The subsequent analytical use of SILAC and TMT proteomic approaches, together with high-sensitivity sample preparation and tailored statistical data analysis, substantially improves RIC's quantitative accuracy and reproducibility. This optimized approach is an extension of the original RIC protocol. It takes 3 d plus 2 weeks for proteomics and data analysis and will enable the study of RBP dynamics under different physiological and pathological conditions.

MATERIALI
N° Catalogo
Marchio
Descrizione del prodotto

Sigma-Aldrich
HEPES, ≥99.5% (titration)
Sigma-Aldrich
Anticorpo anti-β-actina monoclonale murino, clone AC-15, purified from hybridoma cell culture
Millipore
Acido etilendiamminotetraacetico
Sigma-Aldrich
Ribonuclease T1 from Aspergillus oryzae, ammonium sulfate suspension, 300,000-600,000 units/mg protein
Sigma-Aldrich
Ribonucleasi A, Type I-AS, 50-100 Kunitz units/mg protein
Sigma-Aldrich
Monoclonal Anti-PTBP1 antibody produced in mouse, clone 3H8, purified immunoglobulin, buffered aqueous solution