RNA-binding protein IGF2BP3 targeting of oncogenic transcripts promotes hematopoietic progenitor proliferation
Jayanth Kumar Palanichamy, … , Jeremy R. Sanford, Dinesh S. Rao
Jayanth Kumar Palanichamy, … , Jeremy R. Sanford, Dinesh S. Rao
Published March 14, 2016
Citation Information: J Clin Invest. 2016;126(4):1495-1511. https://doi.org/10.1172/JCI80046.
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Research Article Hematology

RNA-binding protein IGF2BP3 targeting of oncogenic transcripts promotes hematopoietic progenitor proliferation

Abstract

Posttranscriptional control of gene expression is important for defining both normal and pathological cellular phenotypes. In vitro, RNA-binding proteins (RBPs) have recently been shown to play important roles in posttranscriptional regulation; however, the contribution of RBPs to cell specification is not well understood. Here, we determined that the RBP insulin-like growth factor 2 mRNA-binding protein 3 (IGF2BP3) is specifically overexpressed in mixed lineage leukemia–rearranged (MLL-rearranged) B-acute lymphoblastic leukemia (B-ALL), which constitutes a subtype of this malignancy associated with poor prognosis and high risk of relapse. IGF2BP3 was required for the survival of B-ALL cell lines, as knockdown led to decreased proliferation and increased apoptosis. Enforced expression of IGF2BP3 provided murine BM cells with a strong survival advantage, led to proliferation of hematopoietic stem and progenitor cells, and skewed hematopoietic development to the B cell/myeloid lineage. Cross-link immunoprecipitation and high throughput sequencing uncovered the IGF2BP3-regulated transcriptome, which includes oncogenes MYC and CDK6 as direct targets. IGF2BP3 regulated transcripts via targeting elements within 3′ untranslated regions (3′UTR), and enforced IGF2BP3 expression in mice resulted in enhanced expression of Myc and Cdk6 in BM. Together, our data suggest that IGF2BP3-mediated targeting of oncogenic transcripts may represent a critical pathogenetic mechanism in MLL-rearranged B-ALL and support IGF2BP3 and its cognate RNA-binding partners as potential therapeutic targets in this disease.

Authors

Jayanth Kumar Palanichamy, Tiffany M. Tran, Jonathan M. Howard, Jorge R. Contreras, Thilini R. Fernando, Timothy Sterne-Weiler, Sol Katzman, Masoud Toloue, Weihong Yan, Giuseppe Basso, Martina Pigazzi, Jeremy R. Sanford, Dinesh S. Rao

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Figure 6

iCLIP analysis of IGF2BP3 in human leukemia cell lines.

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iCLIP analysis of IGF2BP3 in human leukemia cell lines. (A) Proportion o...
(A) Proportion of IGF2BP3 (REH and RS4;11 cells), hnRNPA1(HEK cells), and simulated (Genome) cross-linking sites observed in exons, introns, or unannotated regions of the human genome. (B) Proportion of IGF2BP3 (REH and RS4;11 cells), hnRNPA1 (HEK cells), and simulated (mRNA background) binding sites in coding and noncoding exons. (C) Tetramer sequence enrichment at IGF2BP3–cross-linking sites in RS4;11 and REH cells (upper and lower panel, respectively). (D) IGF2BP3 (REH, RS4;11) and hnRNPA1 (HEK cells) cross-link site density relative to termination codons. (E) IGF2BP3 cross-linking density from REH (dark blue line) and RS4;11 (light blue line) cell lines mapped relative to annotated miR target sites. hnRNPA1 (black line) cross-linking sites from HEK293 cells are included as a control. (F and G) UCSC Genome Browser snapshot of the CDK6 and MYC 3′UTR loci, respectively. Each panel shows the exon-intron structure of the gene, sequence conservation across vertebrate species, and unique read coverage from 2 iCLIP replicates from each cell line. The maximum number of reads at each position is indicated to the left of each histogram. See also Supplemental Figures 5 and 6. (H) Western blot of protein samples from IGF2BP3 RIP. Input refers to RS4;11 cell lysate used for immunoprecipitation. FT is flowthrough of immunoprecipitation from either control (mouse IgG) or IGF2BP3 RIP. RIP is RNA immunoprecipitation from control (mouse IgG) or α-IGF2BP3 antibody (D-7). (I) Scatter bar plots comparing the fold-enrichment for MYC (n = 4, t test; **P < 0.01) and CDK6 (n = 3, t test; *P < 0.05) in control (mouse IgG) and α-IGF2BP3 antibody RNA immunoprecipitations. Levels of MYC and CDK6 are normalized to input levels from total RNA with 18s rRNA as reference.