LMO2 intron 1 mutations in pediatric and adult human T-ALL. (A) LMO2 expression as determined by qRT-PCR in LMO2 translocated T-ALL cell lines (KOPT-K1 and P12-Ichikawa) and nontranslocated T-ALL cell lines (DU.528, PF-382, Loucy, DND41, Jurkat, and ALL-SIL). (B) ChIP-Seq tracks at the LMO2 locus for MYB and H3K27ac in PF-382, DU.528, Loucy, and Jurkat T-ALL cell lines. Y-axis values are reads per bin per million mapped reads. Mutations are shown below as identified by Sanger sequencing of PF-382 and DU.528 DNA, with inserted sequences shown in red and MYB motifs underlined. The position weight matrices for the primary and secondary MYB binding sites are from UniPROBE.²⁷  (C) Pie chart summarizing the percentage of LMO2 transcripts identified by rapid amplification of 5′ complementary DNA ends that start from the distal, intermediate, and proximal promoters for the PF-382, DU.528, and Loucy T-ALL cell lines. A total of 20, 21, and 22 LMO2 transcripts was examined for PF-382, DU.528, and Loucy T-ALL cell lines, respectively. (D) Pie chart summarizing mutation recurrence within pediatric and adult human T-ALL cohorts. (E) Indels mapped to the LMO2 intron 1 mutation hotspot labeled with the associated de novo consensus site as aligned to the UniPROBE or HOCOMOCO position weight matrices, in which MYB, ETS1, and RUNX1 sites are marked as a triangle, square, and diamond, respectively. Below, motif analysis of the region shows the native binding sites for members of the TAL1 complex, including RUNX1, E-box (for TAL1 binding), ETS1, MYB, and GATA. TSS, transcription start site.