Saltar al contenido
Merck

RNase-assisted RNA chromatography.

RNA (New York, N.Y.) (2010-06-24)
Gracjan Michlewski, Javier F Cáceres
RESUMEN

RNA chromatography combined with mass spectrometry represents a widely used experimental approach to identify RNA-binding proteins that recognize specific RNA targets. An important drawback of most of these protocols is the high background due to direct or indirect nonspecific binding of cellular proteins to the beads. In many cases this can hamper the detection of individual proteins due to their low levels and/or comigration with contaminating proteins. Increasing the salt concentration during washing steps can reduce background, but at the cost of using less physiological salt concentrations and the likely loss of important RNA-binding proteins that are less stringently bound to a given RNA, as well as the disassembly of protein or ribonucleoprotein complexes. Here, we describe an improved RNA chromatography method that relies on the use of a cocktail of RNases in the elution step. This results in the release of proteins specifically associated with the RNA ligand and almost complete elimination of background noise, allowing a more sensitive and thorough detection of RNA-binding proteins recognizing a specific RNA transcript.

MATERIALES
Referencia del producto
Marca
Descripción del producto

Sigma-Aldrich
Anti-hnRNP-L antibody, Mouse monoclonal, clone 4D11, purified from hybridoma cell culture