Ribo-proteomics approach to profile RNA–protein and protein–protein interaction networks

Hsin Sung Yeh; Jae Woong Chang; Jeongsik Yong

doi:10.1007/978-1-4939-3591-8_14

Ribo-proteomics approach to profile RNA–protein and protein–protein interaction networks

Hsin Sung Yeh, Jae Woong Chang, Jeongsik Yong

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4 Scopus citations

Abstract

Characterizing protein–protein and protein–RNA interaction networks is a fundamental step to understanding the function of an RNA-binding protein. In many cases, these interactions are transient and highly dynamic. Therefore, capturing stable as well as transient interactions in living cells for the identification of protein-binding partners and the mapping of RNA-binding sequences is key to a successful establishment of the molecular interaction network. In this chapter, we will describe a method for capturing the molecular interactions in living cells using formaldehyde as a crosslinker and enriching a specific RNA–protein complex from cell extracts followed by mass spectrometry and Next-Gen sequencing analyses.

Original language	English (US)
Pages (from-to)	165-174
Number of pages	10
Journal	Methods in Molecular Biology
Volume	1421
DOIs	https://doi.org/10.1007/978-1-4939-3591-8_14
State	Published - Jan 1 2016

Keywords

Crosslinking immunoprecipitation
Formaldehyde crosslinking
Mass spectrometry
Next-Gen sequencing
RNA-binding proteins

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title = "Ribo-proteomics approach to profile RNA–protein and protein–protein interaction networks",

abstract = "Characterizing protein–protein and protein–RNA interaction networks is a fundamental step to understanding the function of an RNA-binding protein. In many cases, these interactions are transient and highly dynamic. Therefore, capturing stable as well as transient interactions in living cells for the identification of protein-binding partners and the mapping of RNA-binding sequences is key to a successful establishment of the molecular interaction network. In this chapter, we will describe a method for capturing the molecular interactions in living cells using formaldehyde as a crosslinker and enriching a specific RNA–protein complex from cell extracts followed by mass spectrometry and Next-Gen sequencing analyses.",

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AU - Yeh, Hsin Sung

AU - Chang, Jae Woong

AU - Yong, Jeongsik

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N2 - Characterizing protein–protein and protein–RNA interaction networks is a fundamental step to understanding the function of an RNA-binding protein. In many cases, these interactions are transient and highly dynamic. Therefore, capturing stable as well as transient interactions in living cells for the identification of protein-binding partners and the mapping of RNA-binding sequences is key to a successful establishment of the molecular interaction network. In this chapter, we will describe a method for capturing the molecular interactions in living cells using formaldehyde as a crosslinker and enriching a specific RNA–protein complex from cell extracts followed by mass spectrometry and Next-Gen sequencing analyses.

AB - Characterizing protein–protein and protein–RNA interaction networks is a fundamental step to understanding the function of an RNA-binding protein. In many cases, these interactions are transient and highly dynamic. Therefore, capturing stable as well as transient interactions in living cells for the identification of protein-binding partners and the mapping of RNA-binding sequences is key to a successful establishment of the molecular interaction network. In this chapter, we will describe a method for capturing the molecular interactions in living cells using formaldehyde as a crosslinker and enriching a specific RNA–protein complex from cell extracts followed by mass spectrometry and Next-Gen sequencing analyses.

KW - Crosslinking immunoprecipitation

KW - Formaldehyde crosslinking

KW - Mass spectrometry

KW - Next-Gen sequencing

KW - RNA-binding proteins

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Ribo-proteomics approach to profile RNA–protein and protein–protein interaction networks

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Keywords

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