The Construction and Verification of CREBBP-m~6A Report System

GUO Jiayin;HUANG Tao;ZENG Wenxian;College of Animal Science and Technology,Northwest A&F University;

GUO Jiayin%HUANG Tao%ZENG Wenxian%College of Animal Science and Technology,Northwest A&F University

N6-methyladenosine(m6A);;RNA modification;;CREBBP-m6A

N6-methyladenosine(m~6A)is the most abundant post-transcription modificational in eukaryotic mRNAs.This dynamic RNA modification has been demonstrated to be regulated by methyltransferase complex and demethylases.M6 A could be recognized by m~6A readers which regulates cellular RNA metabolism including splicing,degradation and translation of target mRNAs.In this study,we constructed CREBBP-m~6A reporter by inserting fragment of CREBBP 3'UTR containing three m~6A motif into downstream of mCherry in pCD513 B-CMV vector,then construct the acquired mCherry-CREBBP 3'UTR fragment in to the pCD513 B-CMV vector between EcoRI and BamHI enzyme cutting cites,and validate the expression of mCherry in GC-1 and 293 Tcells.It was found red fluorescence intensity was negatively related to m~6A level.Results show that CREBBP 3'UTR could regulate target mRNA expression,and CREBBPm~6A reporter could be used to real-timely the change of m~6A modification in cells through expression of mCherry.