Protocol to study the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using cross-linking immunoprecipitation

Clara Bonnet; Ana Luisa Dian; Mélissa Leriche; Patricia Uguen; Stéphan Vagner

doi:10.1016/j.xpro.2024.103292

Protocol to study the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using cross-linking immunoprecipitation

Clara Bonnet
, Ana Luisa Dian
, Mélissa Leriche
, Patricia Uguen
, Stéphan Vagner

Institut Curie
Centre Universitaire
Équipe Labellisée Ligue Contre le Cancer

Résultats de recherche: Contribution à un journal › Article › Revue par des pairs

Résumé

RNA-binding proteins (RBPs) are involved in many biological processes. The direct interaction between protein and RNA can be studied using cross-linking immunoprecipitation (CLIP) techniques in living cells. Here, we present a protocol to characterize the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using CLIP. We describe steps for RNA-protein UV-C crosslinking in living cells, isolating RNA-protein complexes, RNA labeling, and extracting nucleic acid. We then detail procedures for nuclease treatment and nucleic acid migration.

langue originale	Anglais
Numéro d'article	103292
journal	STAR Protocols
Volume	5
Numéro de publication	3
Les DOIs	https://doi.org/10.1016/j.xpro.2024.103292
état	Publié - 20 sept. 2024
Modification externe	Oui

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10.1016/j.xpro.2024.103292

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title = "Protocol to study the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using cross-linking immunoprecipitation",

abstract = "RNA-binding proteins (RBPs) are involved in many biological processes. The direct interaction between protein and RNA can be studied using cross-linking immunoprecipitation (CLIP) techniques in living cells. Here, we present a protocol to characterize the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using CLIP. We describe steps for RNA-protein UV-C crosslinking in living cells, isolating RNA-protein complexes, RNA labeling, and extracting nucleic acid. We then detail procedures for nuclease treatment and nucleic acid migration.",

author = "Clara Bonnet and Dian, \{Ana Luisa\} and M{\'e}lissa Leriche and Patricia Uguen and St{\'e}phan Vagner",

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TY - JOUR

T1 - Protocol to study the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using cross-linking immunoprecipitation

AU - Bonnet, Clara

AU - Dian, Ana Luisa

AU - Leriche, Mélissa

AU - Uguen, Patricia

AU - Vagner, Stéphan

PY - 2024/9/20

Y1 - 2024/9/20

N2 - RNA-binding proteins (RBPs) are involved in many biological processes. The direct interaction between protein and RNA can be studied using cross-linking immunoprecipitation (CLIP) techniques in living cells. Here, we present a protocol to characterize the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using CLIP. We describe steps for RNA-protein UV-C crosslinking in living cells, isolating RNA-protein complexes, RNA labeling, and extracting nucleic acid. We then detail procedures for nuclease treatment and nucleic acid migration.

AB - RNA-binding proteins (RBPs) are involved in many biological processes. The direct interaction between protein and RNA can be studied using cross-linking immunoprecipitation (CLIP) techniques in living cells. Here, we present a protocol to characterize the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using CLIP. We describe steps for RNA-protein UV-C crosslinking in living cells, isolating RNA-protein complexes, RNA labeling, and extracting nucleic acid. We then detail procedures for nuclease treatment and nucleic acid migration.

U2 - 10.1016/j.xpro.2024.103292

DO - 10.1016/j.xpro.2024.103292

M3 - Article

C2 - 39264804

AN - SCOPUS:85205083403

SN - 2666-1667

VL - 5

JO - STAR Protocols

JF - STAR Protocols

IS - 3

M1 - 103292

ER -

Protocol to study the direct binding of proteins to RNA:DNA hybrids or RNA-DNA chimeras in living cells using cross-linking immunoprecipitation

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