Dual-Luciferase Reporter Assay for m6A Site

For dual-luciferase reporter assay, the wild-type and mutated sequence of m⁶A site were designed and synthesized (Supplementary Table 2). The sequences constructed were cloned into pmirGlo luciferase expression vector (Promega, Madison, USA) which were further verified by DNA sequencing. All the specific operations were performed as our previous study [33 (link)].

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Shen H., Ying Y., Ma X., Xie H., Chen S., Sun J., Liu Z., Wen C., Yang Z., Wang X., Xu M., Luo J., Liu B., Li J., Zheng X, & Xie L. (2022). FTO promotes clear cell renal cell carcinoma progression via upregulation of PDK1 through an m6A dependent pathway. Cell Death Discovery, 8, 356.

Publication 2022

pmirGlo luciferase expression vector

Assay Luciferase Promega Vector

Corresponding Organization :

Other organizations : First Affiliated Hospital Zhejiang University, Zhejiang University

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Variable analysis

independent variables

Wild-type m6A site sequence
Mutated m6A site sequence

dependent variables

Luciferase expression

control variables

Luciferase expression vector (pmirGlo)

controls

Positive control: Not specified
Negative control: Not specified

Annotations

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