TY - JOUR
T1 - Transcriptome-wide mapping of N6-methyladenosine by m 6A-seq based on immunocapturing and massively parallel sequencing
AU - Dominissini, Dan
AU - Moshitch-Moshkovitz, Sharon
AU - Salmon-Divon, Mali
AU - Amariglio, Ninette
AU - Rechavi, Gideon
N1 - Funding Information:
acknoWledGMents We thank the Kahn Family Foundation for their support. This work was supported in part by grants from the Flight Attendant Medical Research Institute (FAMRI), Bio-Med Morasha Israel Science Foundation (ISF) (grant no. 1942/08), ISF (grant no. 1667/12), the molecular basis of human disease I-CORE (Israeli Centers of Research Excellence) and the Israel Ministry of Science and Technology (Scientific Infrastructure Program). G.R. holds the Djerassi Chair in Oncology at the Sackler Faculty of Medicine, Tel Aviv University. This work was performed in partial fulfillment of the requirements for a PhD degree to D.D., Sackler Faculty of Medicine, Tel Aviv University.
PY - 2013/1
Y1 - 2013/1
N2 - N6-methyladenosine-sequencing (m6A-seq) is an immunocapturing approach for the unbiased transcriptome-wide localization of m6A in high resolution. To our knowledge, this is the first protocol to allow a global view of this ubiquitous RNA modification, and it is based on antibody-mediated enrichment of methylated RNA fragments followed by massively parallel sequencing. Building on principles of chromatin immunoprecipitation- sequencing (ChIP-seq) and methylated DNA immunoprecipitation (MeDIP), read densities of immunoprecipitated RNA relative to untreated input control are used to identify methylated sites. A consensus motif is deduced, and its distance to the point of maximal enrichment is assessed; these measures further corroborate the success of the protocol. Identified locations are intersected in turn with gene architecture to draw conclusions regarding the distribution of m 6A between and within gene transcripts. When applied to human and mouse transcriptomes, m6A-seq generated comprehensive methylation profiles revealing, for the first time, tenets governing the nonrandom distribution of m6A. The protocol can be completed within ~9 d for four different sample pairs (each consists of an immunoprecipitation and corresponding input).
AB - N6-methyladenosine-sequencing (m6A-seq) is an immunocapturing approach for the unbiased transcriptome-wide localization of m6A in high resolution. To our knowledge, this is the first protocol to allow a global view of this ubiquitous RNA modification, and it is based on antibody-mediated enrichment of methylated RNA fragments followed by massively parallel sequencing. Building on principles of chromatin immunoprecipitation- sequencing (ChIP-seq) and methylated DNA immunoprecipitation (MeDIP), read densities of immunoprecipitated RNA relative to untreated input control are used to identify methylated sites. A consensus motif is deduced, and its distance to the point of maximal enrichment is assessed; these measures further corroborate the success of the protocol. Identified locations are intersected in turn with gene architecture to draw conclusions regarding the distribution of m 6A between and within gene transcripts. When applied to human and mouse transcriptomes, m6A-seq generated comprehensive methylation profiles revealing, for the first time, tenets governing the nonrandom distribution of m6A. The protocol can be completed within ~9 d for four different sample pairs (each consists of an immunoprecipitation and corresponding input).
UR - https://www.scopus.com/pages/publications/84872032385
U2 - 10.1038/nprot.2012.148
DO - 10.1038/nprot.2012.148
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C2 - 23288318
AN - SCOPUS:84872032385
SN - 1754-2189
VL - 8
SP - 176
EP - 189
JO - Nature Protocols
JF - Nature Protocols
IS - 1
ER -