Figure 3. Depletion of PCIF1 distinguishes m⁶A and m⁶Am in transcriptome-wide 6mA maps.

A. Metagene of miCLIP reads in wild-type and PCIF1 knockout (KO) HEK293T cells. Shown is a metagene analysis of reads from the wild-type or PCIF1 KO miCLIP dataset. The first nucleotide of each read (with respect to the RNA strand) was extracted and plotted. Reads in the 5′UTR were lost in the PCIF1 knockout, suggesting a complete loss of m⁶Am in the PCIF1 knockout cells.

B. DREME motif search within called peaks show the DRACH motif as the most enriched in all datasets, consistent m⁶A as the most abundant 6mA-containing nucleotide mapped by miCLIP.

C. miCLIP peaks can be identified as m⁶Am or m⁶A based on their decrease in PCIF1 KO cells. Genome tracks were plotted for RPL35 and KDELR2 with called m⁶A sites (FDR<0.1) and m⁶Am sites indicated by red circles and blue triangle, respectively. Zoomed insets show m⁶Am peaks can be distinguished from nearby m⁶A sites.

D. The previously annotated m⁶Am site in RACK1 is actually a 5′UTR m⁶A. The TSS-proximal peak in RACK1 is not affected in the PCIF1 knockout and overlaps with a DRACH motif.

E. Metagene analysis of PCIF1 KO-validated m⁶Am sites shows m⁶Am sites throughout the 5′UTR and in the transcript body. Shown is a metagene of the exact sites of m⁶Am within the PCIF1-dependent peaks as determined by A to T transitions and the read drop-off method. The metagene reveals an overall enrichment at the TSS, with some sites that appear to be within the CDS and 3′UTR.

F. DREME motif search of the nucleotides surrounding each m⁶Am was performed confirms the previously reported BCA motif, and shows that the promoter sequence upstream of the m⁶Am is GC-enriched.

See also Figure S2.