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. 2020 Apr 3;40(4):BSR20194352. doi: 10.1042/BSR20194352

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© 2020 The Author(s).

This is an open access article published by Portland Press Limited on behalf of the Biochemical Society and distributed under the Creative Commons Attribution License 4.0 (CC BY).

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(A) Predicted mRNAs were showed by Venn diagram. (B) CBX5, TAOK1 and TRAF4 expressions in ESCC tissues. (C) The expressions of CBX5, TAOK1 and TRAF4 in ESCC cells transfected with miR-3612 mimics. (D) TRAF4 expression in ESCC cells and HET-1A cell. (E) The potential interaction between TRAF4 and miR-3612 was validated by RNA pull-down assay. (F) RIP assay was conducted for measuring the binding between TRAF4 and miR-3612. (G) Predicted binding site of miR-3612 on TRAF4. (H) Luciferase activity of TRAF4-WT or TRAF4-MUT was estimated in ESCC cells with the transfection of miR-3612 mimics or NC mimics. (I) Transfection efficiency of pcDNA-TRAF4 in ESCC cells was detected. (J and K) Cell proliferation and apoptosis were determined by transfecting miR-3612 mimics. (L and M) Function of up-regulated miR-3612 on cell migration and invasion; *P <0.05, **P <0.01.