Synergistic roles of DYRK1A and GATA1 in trisomy 21 megakaryopoiesis
Ying Ting Sit, Kaoru Takasaki, Hyun Hyung An, Yan Xiao, Christian Hurtz, Peter A. Gearhart, Zhe Zhang, Paul Gadue, Deborah L. French, Stella T. Chou
Ying Ting Sit, Kaoru Takasaki, Hyun Hyung An, Yan Xiao, Christian Hurtz, Peter A. Gearhart, Zhe Zhang, Paul Gadue, Deborah L. French, Stella T. Chou
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Research Article Hematology

Synergistic roles of DYRK1A and GATA1 in trisomy 21 megakaryopoiesis

Abstract

Patients with Down syndrome (DS), or trisomy 21 (T21), are at increased risk of transient abnormal myelopoiesis (TAM) and acute megakaryoblastic leukemia (ML-DS). Both TAM and ML-DS require prenatal somatic mutations in GATA1, resulting in the truncated isoform GATA1s. The mechanism by which individual chromosome 21 (HSA21) genes synergize with GATA1s for leukemic transformation is challenging to study, in part due to limited human cell models with wild-type GATA1 (wtGATA1) or GATA1s. HSA21-encoded DYRK1A is overexpressed in ML-DS and may be a therapeutic target. To determine how DYRK1A influences hematopoiesis in concert with GATA1s, we used gene editing to disrupt all 3 alleles of DYRK1A in isogenic T21 induced pluripotent stem cells (iPSCs) with and without the GATA1s mutation. Unexpectedly, hematopoietic differentiation revealed that DYRK1A loss combined with GATA1s leads to increased megakaryocyte proliferation and decreased maturation. This proliferative phenotype was associated with upregulation of D-type cyclins and hyperphosphorylation of Rb to allow E2F release and derepression of its downstream targets. Notably, DYRK1A loss had no effect in T21 iPSCs or megakaryocytes with wtGATA1. These surprising results suggest that DYRK1A and GATA1 may synergistically restrain megakaryocyte proliferation in T21 and that DYRK1A inhibition may not be a therapeutic option for GATA1s-associated leukemias.

Authors

Ying Ting Sit, Kaoru Takasaki, Hyun Hyung An, Yan Xiao, Christian Hurtz, Peter A. Gearhart, Zhe Zhang, Paul Gadue, Deborah L. French, Stella T. Chou

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Figure 6

Increased expression of proliferative genes in T21/GATA1s/DYRK1A–/–/– megakaryocytes.

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Increased expression of proliferative genes in T21/GATA1s/DYRK1A–/–/– me...
(A) Representative Western blot analysis of day 4 T21/wtGATA1 or T21/GATA1s megakaryocytes with DYRK1A WT (+/+/+) or knockout (–/–/–) for DYRK1A and cell cycle–related proteins. (B and D) Phosphorylation of cyclin D2 (pT280) and (C) cyclin D3 (pT283) quantified by Western blot band intensity and normalized to total cyclin D2 or D3 expression. n = 3–4 independent experiments per genotype. Data represent the mean ± SEM. Statistical significance was determined by 2-tailed, unpaired t test. *P ≤ 0.05, **P ≤ 0.01. (E) Representative Western blot analysis of day 4 T21/wtGATA1 or T21/GATA1s megakaryocytes with DYRK1A WT (+/+/+) or knockout (–/–/–) for phosphorylated (pRb), hypophosphorylated (hypo-pRb), and total Rb, and (F) GATA1 and GATA2.