Notch Signaling Requires GATA-2 to Inhibit Myelopoiesis from Embryonic Stem Cells and Primary Hemopoietic Progenitors

Pooter, Renée F. de; Schmitt, Thomas M.; Pompa, José Luis de la; Fujiwara, Yuko; Orkin, Stuart H.; Zúñiga‐Pflücker, Juan Carlos

doi:10.4049/jimmunol.176.9.5267

Cited by 62 publications

(63 citation statements)

References 80 publications

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“…In contrast, high levels of either Dll1 or Dll4 effectively inhibited the generation of CD11b + myeloid-lineage cells, similar to that observed in Fig. 1 and as previously reported (15). However, when OP9 cells expressed Dll at medium levels, we noted a clear increase in the generation of myeloid cells as compared with either low or high levels (Fig.…”

Section: B Cell and Myeloid Development On Op9-dl Coculturessupporting

confidence: 71%

“…Viable HPCs were subsequently sorted by flow cytometry as CD117 + Sca-1 + cells. (15). Cells were harvested on day 6 for analysis or further passaged onto fresh plates containing OP9 cells and coculture media for analysis on days 9 and 12.…”

Section: Hpcs and Op9 Coculturesmentioning

confidence: 99%

“…We used this strategy to generate OP9-DL1 cells, which could sustain all stages of T cell development from HPCs, while inhibiting B cell and myeloid lineage differentiation (12)(13)(14)(15). Both Dll1 and Dll4 were shown to be expressed in TECs (16,17), and this initially suggested that there could be redundancy between Dll1 and Dll4 function.…”

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confidence: 99%

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Direct Comparison of Dll1- and Dll4-Mediated Notch Activation Levels Shows Differential Lymphomyeloid Lineage Commitment Outcomes

Mohtashami

Shah

Nakase

et al. 2010

The Journal of Immunology

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141

148

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In the thymus, Notch signaling is essential for T lymphopoiesis, with Delta-like (Dll)4 uniquely involved in this process. However, using cocultures, either Dll4 or Dll1 were shown to support T lymphopoiesis. To address which Dll is more effective at inducing hematopoietic progenitor cells to give rise to T lineage cells in vitro, we generated OP9 cells expressing a series of incrementally discrete and equivalent levels of Dll1 or Dll4. In keeping with previous findings, OP9 cells expressing high levels of either Dll1 or Dll4 gave rise to T lineage cells with similar efficacy, and prevented the differentiation of B and myeloid-lineage cells. However, at limiting levels, Dll4 maintained its ability to inhibit B lineage choice and induce T lineage commitment and differentiation at lower levels than Dll1. This manifest property of Dll4 is evident despite lower levels of steady-state surface expression than Dll1 on OP9 cells. The heightened effectiveness of Dll4 over Dll1 also corresponded to the induction of Notch target genes, and inhibition of B and myeloid-specific transcription factors. Furthermore, we show that OP9 cells expressing levels of Dll4 equivalent to those present in thymic epithelial cells, as expected, gave rise to T lineage cells, but were also permissive for the differentiation of myeloid cells; whereas, still inhibiting B lymphopoiesis. Our findings show that Dll4 expressed at physiological levels on OP9 cells is functionally distinct from similarly expressed levels of Dll1, illustrating the unique properties of Dll4 in supporting the combined T lineage and specific myeloid-lineage outcomes that underpin its function within the thymus.

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Section: B Cell and Myeloid Development On Op9-dl Coculturessupporting

confidence: 71%

Section: Hpcs and Op9 Coculturesmentioning

confidence: 99%

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Direct Comparison of Dll1- and Dll4-Mediated Notch Activation Levels Shows Differential Lymphomyeloid Lineage Commitment Outcomes

Mohtashami

Shah

Nakase

et al. 2010

The Journal of Immunology

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141

148

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“…After 5 min on ice, the lysates were sedimented by centrifugation, and the supernatant was used as the cytoplasmic extract. The pelleted nuclei were washed, and nuclear proteins were extracted with 2 packed cell volumes of nuclear extract buffer (20 mM HEPES [pH 8.0], 420 mM NaCl, 1.5 mM MgCl 2 , 0.5 mM DTT, 0.2 mM EDTA, and 25% glycerol) at 4°C for 45 min. Soluble material was pelleted, and the supernatant was dialyzed at 4°C for 1 h against Shapiro's buffer D (20 mM HEPES [pH 7.9], 20% glycerol, 100 mM KCl, 2 mM DTT, 0.2 mM EDTA, 0.2 mM EGTA, 0.5 mM phenylmethylsulfonyl fluoride, 0.7 mg/liter pepstatin A, and 0.5 mg/liter leupeptin).…”

Section: Methodsmentioning

confidence: 99%

Rbm15 Modulates Notch-Induced Transcriptional Activation and Affects Myeloid Differentiation

Renda

Wang

et al. 2007

Molecular and Cellular Biology

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RBM15 is the fusion partner with MKL in the t(1;22) translocation of acute megakaryoblastic leukemia. To understand the role of the RBM15-MKL1 fusion protein in leukemia, we must understand the normal functions of RBM15 and MKL. Here, we show a role for Rbm15 in myelopoiesis. Rbm15 is expressed at highest levels in hematopoietic stem cells and at more moderate levels during myelopoiesis of murine cell lines and primary murine cells. Decreasing Rbm15 levels with RNA interference enhances differentiation of the 32DWT18 myeloid precursor cell line. Conversely, enforced expression of Rbm15 inhibits 32DWT18 differentiation. We show that Rbm15 alters Notch-induced HES1 promoter activity in a cell type-specific manner. Rbm15 inhibits Notch-induced HES1 transcription in nonhematopoietic cells but stimulates this activity in hematopoietic cell lines, including 32DWT18 and human erythroleukemia cells. Moreover, the N terminus of Rbm15 coimmunoprecipitates with RBPJ, a critical factor in Notch signaling, and the Rbm15 N terminus has a dominant negative effect, impairing activation of HES1 promoter activity by full-length-Rbm15. Thus, Rbm15 is differentially expressed during hematopoiesis and may act to inhibit myeloid differentiation in hematopoietic cells via a mechanism that is mediated by stimulation of Notch signaling via RBPJ.Acute megakaryoblastic leukemia (AML-M7, also referred to as AMKL) comprises approximately 10% of childhood AML, in which it frequently presents in infants with bone marrow fibrosis and progresses rapidly, with a median survival of 8 months. This phenotype is associated with the t(1;22)(p13; q13) translocation, which was first observed in several infants with AML-M7 (5) and subsequently confirmed by others to be associated almost exclusively with this type of AML (2, 30, 31, 34). The t(1;22) translocation has only very rarely been associated with the AML-M7 cases that occur in association with trisomy 21; in general, AML-M7 with trisomy 21 is nearly always associated with mutations in the GATA1 gene (14, 32). In t(1;22), the breakpoint on chromosome 1p13 is within a gene that has been variably named RBM15 for RNA-binding motif protein 15 and OTT (for one twenty-two translocation), and the breakpoint on chromosome 22 is within the MKL1 gene (also known as MAL or BSAC).The MKL1 gene product is a 4.5-kb transcript that is widely expressed in normal tissues (35) and encodes one of three members of the myocardin family. While these three members, i.e., MKL1, MKL2, and myocardin, are only 35% similar to one another at the protein level, they have several highly conserved domains, including RPEL repeats in the N terminus, a region with a B (basic amino acid) box and a glutamine-rich domain that is involved in binding to serum response factor, a leucine zipper-like domain that plays a role in homo-and heterodimerization, and a C-terminal transactivation domain. These proteins also have a SAP domain that, based on its homology to SAF-B, is predicted to associate with matrix attachment regions of transcrip...

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“…Insufficient GATA2 appears to allow HSCs to enter cell cycle and differentiate, thereby depleting self-renewal capacity (Ezoe et al, 2002;de Pater et al, 2013), while over-expression impairs haematopoiesis by blocking differentiation (Heyworth et al, 1999;Persons et al, 1999;Tipping et al, 2009). Fine-tuning of the balance between self-renewal and differentiation of HSC appears to be a critical function of GATA2, possibly through its role in mediating contact-dependent quiescence signals from the BM niche (de Pooter et al, 2006;Guiu et al, 2013). Direct effects on apoptosis are also thought to be mediated by an interaction of GATA2 with BCL2L1 (BCL-XL) (Rodrigues et al, 2005).…”

Section: Haplo-insufficiency Of Gata2mentioning

confidence: 99%

Haematopoietic and immune defects associated with GATA2 mutation

Collin

2018

Pathology

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SummaryHeterozygous familial or sporadic GATA2 mutations cause a multifaceted disorder, encompassing susceptibility to infection, pulmonary dysfunction, autoimmunity, lymphoedema and malignancy. Although often healthy in childhood, carriers of defective GATA2 alleles develop progressive loss of mononuclear cells (dendritic cells, monocytes, B and Natural Killer lymphocytes), elevated FLT3 ligand, and a 90% risk of clinical complications, including progression to myelodysplastic syndrome (MDS) by 60 years of age. Premature death may occur from childhood due to infection, pulmonary dysfunction, solid malignancy and MDS/acute myeloid leukaemia. GATA2 mutations include frameshifts, amino acid substitutions, insertions and deletions scattered throughout the gene but concentrated in the region encoding the two zinc finger domains. Mutations appear to cause haplo-insufficiency, which is known to impair haematopoietic stem cell survival in animal models. Management includes genetic counselling, prevention of infection, cancer surveillance, haematopoietic monitoring and, ultimately, stem cell transplantation upon the development of MDS or another lifethreatening complication.

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Notch Signaling Requires GATA-2 to Inhibit Myelopoiesis from Embryonic Stem Cells and Primary Hemopoietic Progenitors

Cited by 62 publications

References 80 publications

Direct Comparison of Dll1- and Dll4-Mediated Notch Activation Levels Shows Differential Lymphomyeloid Lineage Commitment Outcomes

Direct Comparison of Dll1- and Dll4-Mediated Notch Activation Levels Shows Differential Lymphomyeloid Lineage Commitment Outcomes

Rbm15 Modulates Notch-Induced Transcriptional Activation and Affects Myeloid Differentiation

Haematopoietic and immune defects associated with GATA2 mutation

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