Your search keyword '"Dzierzak, E.A. (Elaine)"' showing total 41 results

1. Rapid Mast Cell Generation from Gata2 Reporter Pluripotent Stem Cells

Author

Kauts, M.-L. (Mari-Liis), De Leo, B. (Bianca), Rodríguez-Seoane, C. (Carmen), Ronn, R. (Roger), Glykofrydis, F. (Fokion), Maglitto, A. (Antonio), Kaimakis, P. (Polynikis), Basi, M. (Margarita), Taylor, H. (Helen), Forrester, L. (Lesley), Wilkinson, A.C. (Adam C.), Göttgens, B. (Berthold), Saunders, P.T. (Philippa TK), Dzierzak, E.A. (Elaine), Kauts, M.-L. (Mari-Liis), De Leo, B. (Bianca), Rodríguez-Seoane, C. (Carmen), Ronn, R. (Roger), Glykofrydis, F. (Fokion), Maglitto, A. (Antonio), Kaimakis, P. (Polynikis), Basi, M. (Margarita), Taylor, H. (Helen), Forrester, L. (Lesley), Wilkinson, A.C. (Adam C.), Göttgens, B. (Berthold), Saunders, P.T. (Philippa TK), and Dzierzak, E.A. (Elaine)

Abstract

Mast cells are tissue-resident immune cells. Their overgrowth/overactivation results in a range of common distressing, sometimes life-threatening disorders, including asthma, psoriasis, anaphylaxis, and mastocytosis. Currently, drug discovery is hampered by use of cancer-derived mast cell lines or primary cells. Cell lines provide low numbers of mature mast cells and are not representative of in vivo mast cells. Mast cell generation from blood/bone marrow gives poor reproducibility, requiring 8-12 weeks of culture. Here we report a method for the rapid/robust production of mast cells from pluripotent stem cells (PSCs). An advantageous Gata2Venus reporter enriches mast cells and progenitors as they differentiate from PSCs. Highly proliferative mouse mast cells and progenitors emerge after 2 weeks. This method is applicable for rapid human mast cell generation, and could enable the production of sufficient numbers of physiologically relevant human mast cells from patient induced PSCs for the study of mast cell-associated disorders and drug discovery.

Published

2018

2. In vivo single cell analysis reveals Gata2 dynamics in cells transitioning to hematopoietic fate

Author

Eich, C. (Christina), Arlt, J. (Jochen), Vink, C.S. (Chris), Solaimani Kartalaei, P. (Parham), Kaimakis, P. (Polynikis), Mariani, S.A. (Samanta A.), Linden, R. (Reinier van der), Cappellen, W.A. (Gert) van, Dzierzak, E.A. (Elaine), Eich, C. (Christina), Arlt, J. (Jochen), Vink, C.S. (Chris), Solaimani Kartalaei, P. (Parham), Kaimakis, P. (Polynikis), Mariani, S.A. (Samanta A.), Linden, R. (Reinier van der), Cappellen, W.A. (Gert) van, and Dzierzak, E.A. (Elaine)

Abstract

Cell fate is established through coordinated gene expression programs in individual cells. Regulatory networks that include the Gata2 transcription factor play central roles in hematopoietic fate establishment. Although Gata2 is essential to the embryonic development and function of hematopoietic stem cells that form the adult hierarchy, little is known about the in vivo expression dynamics of Gata2 in single cells. Here, we examine Gata2 expression in single aortic cells as they establish hematopoietic fate in Gata2Venus mouse embryos. Time-lapse imaging reveals rapid pulsatile level changes in Gata2 reporter expression in cells undergoing endothelial-to-hematopoietic transition. Moreover, Gata2 reporter pulsatile expression is dramatically altered in Gata2+/- aortic cells, which undergo fewer transitions and are reduced in hematopoietic potential. Our novel finding of dynamic pulsatile expression of Gata2 suggests a highly unstable genetic state in single cells concomitant with their transition to hematopoietic fate. This reinforces the notion that threshold levels of Gata2 influence fate establishment and has implications for transcription factor-related hematologic dysfunctions.

Published

2018

3. In Vitro Differentiation of Gata2 and Ly6a Reporter Embryonic Stem Cells Corresponds to In Vivo Waves of Hematopoietic Cell Generation

Author

Kauts, M.-L. (Mari-Liis), Rodriguez-Seoane, C. (Carmen), Kaimakis, P. (Polynikis), Mendes, S.C. (Sandra), Cortés-Lavaud, X. (Xabier), Hill, U. (Undine), Dzierzak, E.A. (Elaine), Kauts, M.-L. (Mari-Liis), Rodriguez-Seoane, C. (Carmen), Kaimakis, P. (Polynikis), Mendes, S.C. (Sandra), Cortés-Lavaud, X. (Xabier), Hill, U. (Undine), and Dzierzak, E.A. (Elaine)

Abstract

In vivo hematopoietic generation occurs in waves of primitive and definitive cell emergence. Differentiation cultures of pluripotent embryonic stem cells (ESCs) offer an accessible source of hematopoietic cells for blood-related research and therapeutic strategies. However, despite many approaches, it remains a goal to robustly generate hematopoietic progenitor and stem cells (HP/SCs) in vitro from ESCs. This is partly due to the inability to efficiently promote, enrich, and/or molecularly direct hematopoietic emergence. Here, we use Gata2Venus (G2V) and Ly6a(SCA1). GFP (LG) reporter ESCs, derived from well-characterized mouse models of HP/SC emergence, to show that during in vitro differentiation they report emergent waves of primitive hematopoietic progenitor cells (HPCs), definitive HPCs, and B-lymphoid cell potential. These results, facilitated by enrichment of single and double reporter cells with HPC properties, demonstrate that in vitro ESC differentiation approximates the waves of hematopoietic cell generation found in vivo, thus raising possibilities for enrichment of rare ESC-derived HP/SCs. Kauts et al. demonstrate that Gata2Venus, Ly6aGFP, and double reporter expression in differentiating mouse embryonic stem cells (ESCs) discriminates and facilitates enrichment of most hematopoietic progenitors generated in vitro. Sequential waves of ESC-derived reporter cell emergence show increasing hematopoietic lineage potency and approximate the in vivo waves of hematopoietic cell generation found in the mouse embryo.

Published

2017

4. Subregional localization and characterization of Ly6aGFP-expressing hematopoietic cells in the mouse embryonic head

Author

Li, Z. (Zhuan), Vink, C.S. (Chris), Mariani, S.A. (Samanta A.), Dzierzak, E.A. (Elaine), Li, Z. (Zhuan), Vink, C.S. (Chris), Mariani, S.A. (Samanta A.), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic cell generation in the midgestation mouse embryo occurs through the natural transdifferentiation of temporally and spatially restricted set of hemogenic endothelial cells. These cells take on hematopoietic fate in the aorta, vitelline and umbilical arteries and appear as hematopoietic cell clusters that emerge from the vascular wall. Gene

Published

2016

5. Hematopoietic (stem) cell development — how divergent are the roads taken?

Author

Kauts, M.-L. (Mari-Liis), Vink, C.S. (Chris), Dzierzak, E.A. (Elaine), Kauts, M.-L. (Mari-Liis), Vink, C.S. (Chris), and Dzierzak, E.A. (Elaine)

Abstract

The development of the hematopoietic system during early embryonic stages occurs in spatially and temporally distinct waves. Hematopoietic stem cells (HSC), the most potent and self-renewing cells of this system, are produced in the final ‘definitive’ wave of hematopoietic cell generation. In contrast to HSCs in the adult, which differentiate via intermediate progenitor populations to produce functional blood cells, the generation of hematopoietic cells in the embryo prior to HSC generation occurs in the early waves by producing blood cells without intermediate progenitors (such as the ‘primitive’ hematopoietic cells). The lineage relationship between the early hematopoietic cells and the cells giving rise to HSCs, the genetic networks controlling their emergence, and the precise temporal determination of HSC fate remain topics of intense research and debate. This Review article discusses the current knowledge on the step-wise embryonic establishment of the adult hematopoietic system, examines the roles of pivotal intrinsic regulators in this process, and raises questions concerning the temporal onset of HSC fate determination.

Published

2016

6. Functional and molecular characterization of mouse Gata2-independent hematopoietic progenitors

Author

Kaimakis, P. (Polynikis), Pater, E. (Emma) de, Eich, C. (Christina), Solaimani Kartalaei, P. (Parham), Kauts, M.-L. (Mari-Liis), Vink, C.S. (Chris), Van Der Linden, R. (Reinier), Jaegle, M.M. (Martine), Yokomizo, T. (Tomomasa), Meijer, D.N. (Dies), Dzierzak, E.A. (Elaine), Kaimakis, P. (Polynikis), Pater, E. (Emma) de, Eich, C. (Christina), Solaimani Kartalaei, P. (Parham), Kauts, M.-L. (Mari-Liis), Vink, C.S. (Chris), Van Der Linden, R. (Reinier), Jaegle, M.M. (Martine), Yokomizo, T. (Tomomasa), Meijer, D.N. (Dies), and Dzierzak, E.A. (Elaine)

Abstract

The Gata2 transcription factor is a pivotal regulator of hematopoietic cell development and maintenance, highlighted by the fact that Gata2 haploinsufficiency has been identified as the cause of some familial cases of acute myelogenous leukemia/myelodysplastic syndrome and in MonoMac syndrome. Genetic deletion in mice has shown that Gata2 is pivotal to the embryonic generation of hematopoietic stem cells (HSCs) and hematopoietic progenitor cells (HPCs). It functions in the embryo during endothelial cell to hematopoietic cell transition to affect hematopoietic cluster, HPC, and HSC formation. Gata2 conditional deletion and overexpression studies show the importance of Gata2 levels in hematopoiesis, during all developmental stages. Although previous studies of cell populations phenotypically enriched in HPCs and HSCs show expression of Gata2, therehasbeen nodirect study of Gata2 expressing cells during normal hematopoiesis. In this study, we generate a Gata2Venus reporter mouse model with unperturbed Gata2 expression to examine the hematopoietic function and transcriptome of Gata2 expressing and nonexpressing cells. We show that all the HSCs are Gata2 expressing. However, not allHPCs in the aorta, vitellineand umbilical arteries, and fetal liver require or express Gata2. These Gata2-independent HPCs exhibit a different functional output and genetic program, including Ras and cyclic AMP response element-binding protein pathways and other Gata factors, compared with Gata2-dependent HPCs. Our results, indicating that Gata2 is of major importance in programming toward HSC fate but not in all cells with HPC fate, have implications for current reprogramming strategies.

Published

2016

7. BMP and Hedgehog Regulate Distinct AGM Hematopoietic Stem Cells Ex Vivo

Author

Crisan, M. (Mihaela), Solaimani Kartalaei, P. (Parham), Neagu, A. (Alex), Karkanpouna, S. (Sofia), Yamada-Inagawa, T. (Tomoko), Purini, C. (Caterina), Vink, C.S. (Chris), Linden, R. (Reinier) van der, IJcken, W.F.J. (Wilfred) van, Sousa Lopes, S.C. (Susana Chuva) de, Monteiro, R. (Rui), Mummery, C.L. (Christine), Dzierzak, E.A. (Elaine), Crisan, M. (Mihaela), Solaimani Kartalaei, P. (Parham), Neagu, A. (Alex), Karkanpouna, S. (Sofia), Yamada-Inagawa, T. (Tomoko), Purini, C. (Caterina), Vink, C.S. (Chris), Linden, R. (Reinier) van der, IJcken, W.F.J. (Wilfred) van, Sousa Lopes, S.C. (Susana Chuva) de, Monteiro, R. (Rui), Mummery, C.L. (Christine), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic stem cells (HSC), the self-renewing cells of the adult blood differentiation hierarchy, are generated during embryonic stages. The first HSCs are produced in the aorta-gonad-mesonephros (AGM) region of the embryo through endothelial to a hematopoietic transition. BMP4 and Hedgehog affect their production and expansion, but it is unknown whether they act to affect the same HSCs. In this study using the BRE GFP reporter mouse strain that identifies BMP/Smad-activated cells, we find that the AGM harbors two types of adult-repopulating HSCs upon explant culture: One type is BMP-activated and the other is a non-BMP-activated HSC type that is indirectly controlled by Hedgehog signaling through the VEGF pathway. Transcriptomic analyses demonstrate that the two HSC types express distinct but overlapping genetic programs. These results revealing the bifurcation in HSC types at early embryonic stages in the AGM explant model suggest that their development is dependent upon the signaling molecules in the microenvironment.

Published

2016

8. Whole-transcriptome analysis of endothelial to hematopoietic stem cell transition reveals a requirement for Gpr56 in HSC generation

Author

Solaimani Kartalaei, P. (Parham), Yamada-Inagawa, T. (Tomoko), Vink, C.S. (Chris), Pater, E. (Emma) de, Van Der Linden, R. (Reinier), Marks-Bluth, J. (Jonathon), van der Sloot, A. (Anthon), van den hout, M.C.G.N. (Mirjam), Yokomizo, T. (Tomomasa), Lucila van Schaick-Solernó, M. (M.), Delwel, H.R. (Ruud), Pimanda, J.E. (John), IJcken, W.F.J. (Wilfred) van, Dzierzak, E.A. (Elaine), Solaimani Kartalaei, P. (Parham), Yamada-Inagawa, T. (Tomoko), Vink, C.S. (Chris), Pater, E. (Emma) de, Van Der Linden, R. (Reinier), Marks-Bluth, J. (Jonathon), van der Sloot, A. (Anthon), van den hout, M.C.G.N. (Mirjam), Yokomizo, T. (Tomomasa), Lucila van Schaick-Solernó, M. (M.), Delwel, H.R. (Ruud), Pimanda, J.E. (John), IJcken, W.F.J. (Wilfred) van, and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic stem cells (HSCs) are generated via a natural transdifferentiation process known as endothelial to hematopoietic cell transition (EHT). Because of small numbers of embryonal arterial cells undergoing EHT and the paucity of markers to enrich for hemogenic endothelial cells (ECs [HECs]), the genetic program driving HSC emergence is largely unknown. Here, we use a highly sensitive RNAseq method to examine the whole transcriptome of small numbers of enriched aortic HSCs, HECs, and ECs. Gpr56, a G-coupled protein receptor, is one of the most highly up-regulated of the 530 differentially expressed genes. Also, highly up-regulated are hematopoietic transcription factors, including the "heptad" complex of factors. We show that Gpr56 (mouse and human) is a target of the heptad complex and is required for hematopoietic cluster formation during EHT. Our results identify the processes and regulators involved in EHT and reveal the surprising requirement for Gpr56 in generating the first HSCs.

Published

2015

9. BMP signalling differentially regulates distinct haematopoietic stem cell types

Author

Crisan, M. (Mihaela), Solaimani Kartalaei, P. (Parham), Vink, C.S. (Chris), Yamada-Inagawa, T. (Tomoko), Bollerot, K. (Karine), IJcken, W.F.J. (Wilfred) van, Van Der Linden, R. (Reinier), Sousa Lopes, S.C. (Susana Chuva) de, Monteiro, R. (Rui), Mummery, C.L. (Christine), Dzierzak, E.A. (Elaine), Crisan, M. (Mihaela), Solaimani Kartalaei, P. (Parham), Vink, C.S. (Chris), Yamada-Inagawa, T. (Tomoko), Bollerot, K. (Karine), IJcken, W.F.J. (Wilfred) van, Van Der Linden, R. (Reinier), Sousa Lopes, S.C. (Susana Chuva) de, Monteiro, R. (Rui), Mummery, C.L. (Christine), and Dzierzak, E.A. (Elaine)

Abstract

Adult haematopoiesis is the outcome of distinct haematopoietic stem cell (HSC) subtypes with self-renewable repopulating ability, but with different haematopoietic cell lineage outputs. The molecular basis for this heterogeneity is largely unknown. BMP signalling regulates HSCs as they are first generated in the aorta-gonad-mesonephros region, but at later developmental stages, its role in HSCs is controversial. Here we show that HSCs in murine fetal liver and the bone marrow are of two types that can be prospectively isolated - BMP activated and non-BMP activated. Clonal transplantation demonstrates that they have distinct haematopoietic lineage outputs. Moreover, the two HSC types differ in intrinsic genetic programs, thus supporting a role for the BMP signalling axis in the regulation of HSC heterogeneity and lineage output. Our findings provide insight into the molecular control mechanisms that define HSC types and have important implications for reprogramming cells to HSC fate and treatments targeting distinct HSC types.

Published

2015

10. Identification of Cdca7 as a novel Notch transcriptional target involved in hematopoietic stem cell emergence

Author

Guiu, J. (Jordi), Bergen, D.J.M. (Dylan J.M.), Pater, E. (Emma) de, Islam, A.B.M.M.K. (Abul), Ayllón, V. (Verónica), Gama-Norton, L. (Leonor), Ruiz-Herguido, C. (Cristina), González, J. (Jessica), López-Bigas, N. (Núria), Menéndez, P. (Pablo), Dzierzak, E.A. (Elaine), Espinosa, L. (Lluis), Bigas, A. (Anna), Guiu, J. (Jordi), Bergen, D.J.M. (Dylan J.M.), Pater, E. (Emma) de, Islam, A.B.M.M.K. (Abul), Ayllón, V. (Verónica), Gama-Norton, L. (Leonor), Ruiz-Herguido, C. (Cristina), González, J. (Jessica), López-Bigas, N. (Núria), Menéndez, P. (Pablo), Dzierzak, E.A. (Elaine), Espinosa, L. (Lluis), and Bigas, A. (Anna)

Abstract

Hematopoietic stem cell (HSC) specification occurs in the embryonic aorta and requires Notch activation; however, most of the Notch-regulated elements controlling de novo HSC generation are still unknown. Here, we identify putative direct Notch targets in the aorta-gonad-mesonephros (AGM) embryonic tissue by chromatin precipitation using antibodies against the Notch partner RBPj. By ChIP-on-chip analysis of the precipitated DNA, we identified 701 promoter regions that were candidates to be regulated by Notch in the AGM. One of the most enriched regions corresponded to the Cdca7 gene, which was subsequently confirmed to recruit the RBPj factor but also Notch1 in AGM cells. We found that during embryonic hematopoietic development, expression of Cdca7 is restricted to the hematopoietic clusters of the aorta, and it is strongly up-regulated in the hemogenic population during human embryonic stem cell hematopoietic differentiation in a Notchdependent manner. Down-regulation of Cdca7 mRNA in cultured AGM cells significantly induces hematopoietic differentiation and loss of the progenitor population. Finally, using loss-of-function experiments in zebrafish, we demonstrate that CDCA7 contributes to HSC emergence in vivo during embryonic development. Thus, our study identifies Cdca7 as an evolutionary conserved Notch target involved in HSC emergence.

Published

2014

11. The biochemistry of hematopoietic stem cell development

Author

Kaimakis, P. (Polynikis), Crisan, M. (Mihaela), Dzierzak, E.A. (Elaine), Kaimakis, P. (Polynikis), Crisan, M. (Mihaela), and Dzierzak, E.A. (Elaine)

Abstract

Background: The cornerstone of the adult hematopoietic system and clinical treatments for blood-related disease is the cohort of hematopoietic stem cells (HSC) that is harbored in the adult bone marrow microenvironment. Interestingly, this cohort of HSCs is generated only during a short window of developmental time. In mammalian embryos, hematopoietic progenitor and HSC generation occurs within several extra- and intraembryonic microenvironments, most notably from 'hemogenic' endothelial cells lining the major vasculature. HSCs are made through a remarkable transdifferentiation of endothelial cells to a hematopoietic fate that is l

Published

2013

12. Gata2 is required for HSC generation and survival

Author

Pater, E. (Emma) de, Kaimakis, P. (Polynikis), Vink, C.S. (Chris), Yokomizo, T. (Tomomasa), Yamada-Inagawa, T. (Tomoko), Linden, R. (Reinier) van der, Solaimani Kartalaei, P. (Parham), Camper, S.A. (S.), Speck, N.A. (Nancy), Dzierzak, E.A. (Elaine), Pater, E. (Emma) de, Kaimakis, P. (Polynikis), Vink, C.S. (Chris), Yokomizo, T. (Tomomasa), Yamada-Inagawa, T. (Tomoko), Linden, R. (Reinier) van der, Solaimani Kartalaei, P. (Parham), Camper, S.A. (S.), Speck, N.A. (Nancy), and Dzierzak, E.A. (Elaine)

Abstract

Knowledge of the key transcription factors that drive hematopoietic stem cell (HSC) generation is of particular importance for current hematopoietic regenerative approaches and reprogramming strategies. Whereas GATA2 has long been implicated as a hematopoietic transcription factor and its dysregulated expression is associated with human immunodeficiency syndromes and vascular integrity, it is as yet unknown how GATA2 functions in the generation of HSCs. HSCs are generated from endothelial cells of the major embryonic vasculature (aorta, vitelline, and umbilical arteries) and are found in intra-aortic hematopoietic clusters. In this study, we find that GATA2 function is essential for the generation of HSCs during the stage of endothelial-to-hematopoietic cell transition. Specific deletion of Gata2 in Vec (Vascular Endothelial Cadherin)-expressing endothelial cells results in a deficiency of long-term repopulating HSCs and intra-aortic cluster cells. By specific deletion of Gata2 in Vav-expressing hematopoietic cells (after HSC generation), we further show that GATA2 is essential for HSC survival. This is in contrast to the known activity of the RUNX1 transcription factor, which functions only in the generation of HSCs, and highlights the unique requirement for GATA2 function in HSCs throughout all developmental stages.

Published

2013

13. Hes repressors are essential regulators of hematopoietic stem cell development downstream of notch signaling

Author

Guiu, J. (Jordi), Shimizu, R. (Ritsuko), D'Altri, C., Fraser, S.T. (Stuart), Hatakeyama, S. (Shingo), Bresnick, E.H. (Emery), Kageyama, T. (Tsutomu), Dzierzak, E.A. (Elaine), Yamamoto, M. (Masayuki), Espinosa, L. (Lluis), Bigas, A. (Anna), Guiu, J. (Jordi), Shimizu, R. (Ritsuko), D'Altri, C., Fraser, S.T. (Stuart), Hatakeyama, S. (Shingo), Bresnick, E.H. (Emery), Kageyama, T. (Tsutomu), Dzierzak, E.A. (Elaine), Yamamoto, M. (Masayuki), Espinosa, L. (Lluis), and Bigas, A. (Anna)

Abstract

Previous studies have identified Notch as a key regulator of hematopoietic stem cell (HSC) development, but the underlying downstream mechanisms remain unknown. The Notch target Hes1 is widely expressed in the aortic endothelium and hematopoietic clusters, though Hes1-deficient mice show no overt hematopoietic abnormalities. We now demonstrate that Hes is required for the development of HSC in the mouse embryo, a function previously undetected as the result of functional compensation by de novo expression of Hes5 in the aorta/gonad/mesonephros (AGM) region of Hes1 mutants. Analysis of embryos deficient for Hes1 and Hes5 reveals an intact arterial program with overproduction of nonfunctional hematopoietic precursors and total absence of HSC activity. These alterations were associated with increased expression of the hematopoietic regulators Runx1, c-myb, and the previously identified Notch target Gata2. By analyzing the Gata2 locus, we have identified functional RBPJ-binding sites, which mutation results in loss of Gata2 reporter expression in transgenic embryos, and functional Hes-binding sites, which mutation leads to specific Gata2 up-regulation in the hematopoietic precursors. Together, our findings show that Notch activation in the AGM triggers Gata2 and Hes1 transcription, and next HES-1 protein represses Gata2, creating an incoherent feed-forward loop required to restrict Gata2 expression in the emerging HSCs.

Published

2013

14. Erythropoiesis: Development and differentiation

Author

Dzierzak, E.A. (Elaine), Philipsen, J.N.J. (Sjaak), Dzierzak, E.A. (Elaine), and Philipsen, J.N.J. (Sjaak)

Abstract

Through their oxygen delivery function, red blood cells are pivotal to the healthy existence of all vertebrate organisms. These cells are required during all stages of life-embryonic, fetal, neonatal, adolescent, and adult. In the adult, red blood cells are the terminally differentiated end-product cells of a complex hierarchy of hematopoietic progenitors that become progressively restricted to the erythroid lineage. During this stepwise differentiation process, erythroid progenitors undergo enormous expansion, so as to fulfill the daily requirement of ~2 × 1011 new erythrocytes. How the erythroid lineage is made has been a topic of intense research over the last decades. Developmental studies show that there are two types of red blood cells-embryonic and adult. They develop from distinct hemogenic/hematopoietic progenitors in different anatomical sites and show distinct genetic programs. This arti

Published

2013

15. Dlk1 is a negative regulator of emerging hematopoietic stem and progenitor cells

Author

Mirshekar-Syahkal, B. (Bahar), Haak, E. (Esther), Kimber, G.M. (Gillian), Leusden, K. (Kevin) van, Harvey, K. (Kirsten), O'Rourke, R.A., Laborda, J. (Jorge), Bauer, S.R. (Steven), Bruijn, M.F.T.R. (Marella) de, Ferguson-Smith, A. (Anne), Dzierzak, E.A. (Elaine), Ottersbach, K. (Katrin), Mirshekar-Syahkal, B. (Bahar), Haak, E. (Esther), Kimber, G.M. (Gillian), Leusden, K. (Kevin) van, Harvey, K. (Kirsten), O'Rourke, R.A., Laborda, J. (Jorge), Bauer, S.R. (Steven), Bruijn, M.F.T.R. (Marella) de, Ferguson-Smith, A. (Anne), Dzierzak, E.A. (Elaine), and Ottersbach, K. (Katrin)

Abstract

The first mouse adult-repopulating hematopoietic stem cells emerge in the aorta-gonad-mesonephros region at embryonic day (E) 10.5. Their numbers in this region increase thereafter and begin to decline at E12.5, thus pointing to the possible existence of both positive and negative regulators of emerging hematopoietic stem cells. Our recent expression analysis of the aorta-gonad-mesonephros region showed that the Delta-like homologue 1 (Dlk1) gene is up-regulated in the region of the aorta-gonad-mesonephros where hematopoietic stem cells are preferentially located. To analyze its function, we studied Dlk1 expression in wild-type and hematopoietic stem cell-deficient embryos and determined hematopoietic stem and progenitor cell activity in Dlk1 knockout and overexpressing mice. Its role in hematopoietic support was studied in co-culture experiments using stromal cell lines that express varying levels of Dlk1. We show here that Dlk1 is expressed in the smooth muscle layer of the dorsal aorta and the ventral sub-aortic mesenchyme, where its expression is dependent on the hematopoietic transcription factor Runx1. We further demonstrate that Dlk1 has a negative impact on hematopoietic stem and progenitor cell activity in the aorta-gonad-mesonephros region in vivo, which is recapitulated in co-cultures of hematopoietic stem cells on stromal cells that express varying levels of Dlk1. This negative effect of Dlk1 on hematopoietic stem and progenitor cell activity requires the membrane-bound form of the protein and cannot be recapitulated by soluble Dlk1. Together, these data suggest that Dlk1 expression by cells of the aorta-gonad-mesonephros hematopoietic microenvironment limits hematopoietic stem cell expansion and is, to our knowled

Published

2013

16. Whole-mount three-dimensional imaging of internally localized immunostained cells within mouse embryos

Author

Yokomizo, T. (Tomomasa), Yamada-Inagawa, T. (Tomoko), Yzaguirre, A.D. (Amanda), Chen, M.J. (Michael), Speck, N.A. (Nancy), Dzierzak, E.A. (Elaine), Yokomizo, T. (Tomomasa), Yamada-Inagawa, T. (Tomoko), Yzaguirre, A.D. (Amanda), Chen, M.J. (Michael), Speck, N.A. (Nancy), and Dzierzak, E.A. (Elaine)

Abstract

We describe a three-dimensional (3D) confocal imaging technique to characterize and enumerate rare, newly emerging hematopoietic cells located within the vasculature of whole-mount preparations of mouse embryos. However, the methodology is broadly applicable for examining the development and 3D architecture of other tissues. Previously, direct whole-mount imaging has been limited to external tissue layers owing to poor laser penetration of dense, opaque tissue. Our whole-embryo imaging method enables detailed quantitative and qualitative analysis of cells within the dorsal aorta of embryonic day (E) 10.5-11.5 embryos after the removal of only the head and body walls. In this protocol we describe the whole-mount fixation and multimarker staining procedure, the tissue transparency treatment, microscopy and the analysis of resulting images. A typical two-color staining experiment can be performed and analyzed in ∼6 d.

Published

2012

17. Three-dimensional imaging of whole midgestation murine embryos shows an intravascular localization for all hematopoietic clusters

Author

Yokomizo, T. (Tomomasa), Ng, C.E.L., Osato, M. (Motomi), Dzierzak, E.A. (Elaine), Yokomizo, T. (Tomomasa), Ng, C.E.L., Osato, M. (Motomi), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic cell clusters associated with the midgestation mouse aorta, umbilical and vitelline arteries play a pivotal role in the formation of the adult blood system. Both genetic and live-imaging data indicate that definitive hematopoietic progenitor/stem cells (visualized as clusters) are generated from hemogenic endothelium.A3-dimensional (3-D) whole embryo immunostaining and imaging technique has allowed quantitation and cartographic mapping of intravascular hematopoietic clusters. During this period the vitelline artery is most extensively remodeled, and several reports have suggested that vitelline remodeling leads to extravascular hematopoietic cluster emergence. Whether the earliest definitive progenitors/ stem cells are intra or extra vascular could influence the process by which these cells migrate to the next hematopoietic territory, the fetal liver. Hence, by 3-D imaging we more closely examined hematopoietic clusters in the vitelline and associated connected small vessels and show here that hematopoietic clusters (particularly large clusters) are intravascular during the period of vascular remodeling.

Published

2011

18. CD41 is developmentally regulated and differentially expressed on mouse hematopoietic stem cells

Author

Robin, C. (Catherine), Ottersbach, K. (Katrin), Boisset, J.C. (Jean Charles), Oziemlak, A. (Aneta), Dzierzak, E.A. (Elaine), Robin, C. (Catherine), Ottersbach, K. (Katrin), Boisset, J.C. (Jean Charles), Oziemlak, A. (Aneta), and Dzierzak, E.A. (Elaine)

Abstract

CD41 expression is associated with the earliest stages of mouse hematopoiesis. It is notably expressed on some cells of the intra-aortic hematopoietic clusters, an area where the first adult-repopulating hematopoietic stem cells (HSCs) are generated. Although it is generally accepted that CD41 expression marks the onset of primitive/definitive hematopoiesis, there are few published data concerning its expression on HSCs. It is as yet uncertain whether HSCs express CD41 throughout development, and if so, to what level. We performed a complete in vivo transplantation analysis with yolk sac, aorta, placenta, and fetal liver cells, sorted based on CD41 expression level. Our data show that the earliest emerging HSCs in the aorta express CD41 in a time-dependent manner. In contrast, placenta

Published

2011

19. Placenta as a source of hematopoietic stem cells

Author

Dzierzak, E.A. (Elaine), Robin, C. (Catherine), Dzierzak, E.A. (Elaine), and Robin, C. (Catherine)

Abstract

The placenta is a large, highly vascularised hematopoietic tissue that functions during the embryonic and foetal development of eutherian mammals. Although recognised as the interface tissue important in the exchange of oxygen, nutrients and waste products between the foetus and mother, the placenta has increasingly become a focus of research concerning the ontogeny of the blood system. Here, we describe recent data showing the intrinsic hematopoietic potential and appearance of hematopoietic cells in the mouse and human placenta and probe the biological rationale behind its hematopoietic function. As a rest tissue that contains potent hematopoietic stem cells (HSCs), the human placenta could represent (in addition to umbilical cord blood cells) an accessible supplemental source of cells for therapeutic strategies.

Published

2010

20. Three-dimensional cartography of hematopoietic clusters in the vasculature of whole mouse embryos

Author

Yokomizo, T. (Tomomasa), Dzierzak, E.A. (Elaine), Yokomizo, T. (Tomomasa), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic cell clusters in the aorta of vertebrate embryos play a pivotal role in the formation of the adult blood system. Despite their importance, hematopoietic clusters have not been systematically quantitated or mapped because of technical limitations posed by the opaqueness of whole mouse embryos. Here, we combine an approach to make whole mouse embryos transparent, with multicolor marking, to allow observation of hematopoietic clusters using high-resolution 3-dimensional confocal microscopy. Our method provides the first complete map and temporal quantitation of all hematopoietic clusters in the mouse embryonic vasculature. We show that clusters peak in number at embryonic day 10.5, localize to specific vascular subregions and are heterogeneous, indicating a basal endothelial to non-basal (outer cluster) hematopoietic cell transition. Clusters enriched with the c-Kit+CD31+SSEA1-cell population contain functional hematopoietic progenitors and stem cells. Thus, three-dimensional cartography of transparent mouse embryos provides novel insight into the vascular subregions instrumental in hematopoietic progenitor/stem cell development, and represents an important technological advancement for comprehensive in situ hematopoietic cluster analysis.

Published

2010

21. Ventral embryonic tissues and Hedgehog proteins induce early AGM hematopoietic stem cell development

Author

Peeters, M. (Marian), Ottersbach, K. (Katrin), Bollerot, K. (Karine), Orelino, C. (Claudia), Bruijn, M.F.T.R. (Marella) de, Wijgerde, M.G.J.M. (Mark), Dzierzak, E.A. (Elaine), Peeters, M. (Marian), Ottersbach, K. (Katrin), Bollerot, K. (Karine), Orelino, C. (Claudia), Bruijn, M.F.T.R. (Marella) de, Wijgerde, M.G.J.M. (Mark), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoiesis is initiated in several distinct tissues in the mouse conceptus. The aorta-gonad-mesonephros (AGM) region is of particular interest, as it autonomously generates the first adult type hematopoietic stem cells (HSCs). The ventral position of hematopoietic clusters closely associated with the aorta of most vertebrate embryos sug

Published

2009

22. Human Placenta Is a Potent Hematopoietic Niche Containing Hematopoietic Stem and Progenitor Cells throughout Development

Author

Robin, C. (Catherine), Bollerot, K. (Karine), Mendes, S.C. (Sandra), Haak, E. (Esther), Crisan, M. (Mihaela), Cerisoli, F. (Francesco), Lauw, I. (Ivoune), Kaimakis, P. (Polynikis), Jorna, R.J.J. (Ruud), Vermeulen, M. (Mark), Kayser, M.H. (Manfred), Linden, R. (Reinier) van der, Imanirad, P. (Parisa), Verstegen, M.M.A. (Monique), Nawaz-Yousaf, H. (Humaira), Papazian, N. (Natalie), Steegers, E.A.P. (Eric), Cupedo, T. (Tom), Dzierzak, E.A. (Elaine), Robin, C. (Catherine), Bollerot, K. (Karine), Mendes, S.C. (Sandra), Haak, E. (Esther), Crisan, M. (Mihaela), Cerisoli, F. (Francesco), Lauw, I. (Ivoune), Kaimakis, P. (Polynikis), Jorna, R.J.J. (Ruud), Vermeulen, M. (Mark), Kayser, M.H. (Manfred), Linden, R. (Reinier) van der, Imanirad, P. (Parisa), Verstegen, M.M.A. (Monique), Nawaz-Yousaf, H. (Humaira), Papazian, N. (Natalie), Steegers, E.A.P. (Eric), Cupedo, T. (Tom), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic stem cells (HSCs) are responsible for the life-long production of the blood system and are pivotal cells in hematologic transplantation therapies. During mouse and human development, the first HSCs are produced in the aorta-gonad-mesonephros region. Subsequent to this emergence, HSCs are found in other anatomical sites of the mouse conceptus. While the mouse placenta contains abundant HSCs at midgestation, little is known concerning whether HSCs or hematopoietic progenitors are present and supported in the human placenta during development. In this study we show, over a range of developmental times including term, that the human placenta contains hematopoietic progenitors and HSCs. Moreover, stromal cell lines generated from human placenta at several developmental time points are pericyte-like cells and support human hematopoiesis. Immunostaining of placenta sections during development localizes hematopoietic cells in close contact with pericytes/perivascular cells. Thus, the human placenta is a potent hematopoietic niche throughout development.

Published

2009

23. Interleukin-1 regulates Hematopoietic progenitor and stem cells in the midgestation mouse fetal liver

Author

Orelio, C. (Claudia), Peeters, M. (Marian), Haak, E. (Esther), Horn, K. (Karin) van der, Dzierzak, E.A. (Elaine), Orelio, C. (Claudia), Peeters, M. (Marian), Haak, E. (Esther), Horn, K. (Karin) van der, and Dzierzak, E.A. (Elaine)

Abstract

Background Hematopoietic progenitors are generated in the yolk sac and aorta-gonad-mesonephros region during early mouse development. At embryonic day 10.5 the first hematopoietic stem cells emerge in the aorta-gonad-mesonephros. Subsequently, hematopoietic stem cells and progenitors are found in the fetal liver. The fetal liver is a potent hematopoietic site, playing an important role in the expansion and differentiation of hematopoietic progenitors and hematopoietic stem cells. However, little is known concerning the regulation of fetal liver hematopoietic stem cells. In particular, the role of cytokines such as interleukin-1 in the regulation of hematopoietic stem cells in the embryo has been largely unexplored. Recently, we observed that the adult pro-inflammatory cytokine interleukin-1 is involved in regulating aorta-gonad-mesonephros hematopoietic progenitor and hematopoietic stem cell activity. Therefore, we set out to investigate whether interleukin- 1 also plays a role in regulating fetal liver progenitor cells and hematopoietic stem cells. Design and Methods We examined the interleukin-1 ligand and receptor expression pattern in the fetal liver. The effects of interleukin-1 on hematopoietic progenitor cells and hematopoietic stem cells were studied by FACS and tr

Published

2009

24. Opening act in a hematopoietic program

Author

Dzierzak, E.A. (Elaine) and Dzierzak, E.A. (Elaine)

Published

2009

25. Fine-tuning of hematopoietic stem cell homeostasis: Novel role for ubiquitin ligase

Author

Yokomizo, T. (Tomomasa), Dzierzak, E.A. (Elaine), Yokomizo, T. (Tomomasa), and Dzierzak, E.A. (Elaine)

Abstract

Homeostasis of hematopoietic stem cells (HSCs) is a tightly regulated process, controlled by intrinsic and extrinsic signals. Although a variety of molecules involved in HSC maintenance and self-renewal are known, it remains unclear how robust HSC homeostasis is achieved. In this issue of Genes & Development, Rathinam and colleagues (pp. 992-997) report a new player in HSC homeostasis, c-Cbl ubiq-uitin ligase. They show that this E3 ubiquitin ligase acts as a negative regulator of cytokine signaling.

Published

2008

26. Of lineage and legacy: The development of mammalian hematopoietic stem cells

Author

Dzierzak, E.A. (Elaine), Speck, N.A. (Nancy), Dzierzak, E.A. (Elaine), and Speck, N.A. (Nancy)

Abstract

The hematopoietic system is one of the first complex tissues to develop in the mammalian conceptus. Of particular interest in the field of developmental hematopoiesis is the origin of adult bone marrow hematopoietic stem cells. Tracing their origin is complicated because blood is a mobile tissue and because hematopoietic cells emerge from many embryonic sites. The origin of the adult mammalian blood system remains a topic of lively discussion and intense research. Interest is also focused on developmental signals that induce the adult hematopoietic stem cell program, as these may prove useful for generating and expanding these clinically important cell populations ex vivo. This review presents a historical overview of and the most recent data on the developmental origins of hematopoiesis.

Published

2008

27. The discovery of a source of adult hematopoietic cells in the embryo

Author

Dzierzak, E.A. (Elaine), Medvinsky, A. (Alexander), Dzierzak, E.A. (Elaine), and Medvinsky, A. (Alexander)

Abstract

This essay is about the 1975 JEEM paper by Françoise Dieterlen-Lièvre (Dieterlen-Lièvre, 1975) and the studies that followed it, which indicated that the adult hematopoietic system in the avian embryo originates, not from the blood islands of the extraembryonic yolk sac as was then believed, but from the body of the embryo itself. Dieterien-Lièvre's 1975 paper created a paradigm shift in hematopoietic research, and provided a new and lasting focus on hematopoietic activity within the embryo body.

Published

2008

28. Stem cell researchers find their niche

Author

Dzierzak, E.A. (Elaine), Enver, T. (Tariq), Dzierzak, E.A. (Elaine), and Enver, T. (Tariq)

Abstract

The EuroSTELLS Workshop 'Stem Cell Niches', organised by Anna Bigas, Ernest Arenas and Pasqualino Loi, took place in January 2008 in Barcelona, Spain. The goal of the conference was to promote scientific collaboration and synergy between stem cell researchers worldwide and those in the EuroSTELLS consortia (an initiative of the European Science Foundation EUROCORES Programme), and to stimulate discussion of the latest results in the field of stem cell niches.

Published

2008

29. Interleukin-1 mediated hematopoietic cell regulation in the aorta-gonad-mesonephros region of the mouse embryo

Author

Orelio, C. (Claudia), Haak, E. (Esther), Peeters, M. (Marian), Dzierzak, E.A. (Elaine), Orelio, C. (Claudia), Haak, E. (Esther), Peeters, M. (Marian), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoiesis during development is a dynamic process, with many factors involved in the emergence and regulation of hematopoietic stem cells (HSCs) and progenitor cells. Whereas previous studies have focused on developmental signaling and transcription factors in embryonic hematopoiesis, the role of well-known adult hematopoietic cytokines in the embryonic hematopoietic system has been largely unexplored. The cytokine interleukin-1 (IL-1), best known for its proinflammatory properties, has radiopro-tective effects on adult bone marrow HSCs, induces HSC mobilization, and increases HSC proliferation and/or differentiation. Here we examine IL-1 and its possible role in regulating hematopoiesis in the midgestation mouse embryo. We show that IL-1, IL-1 receptors (IL-1Rs), and signaling mediators are expressed in the aorta-gonad-mesonephros (AGM) region during the time when HSCs emerge in this site. IL-1 signaling is functional in the AGM, and the IL-1RI is expressed ventrally in the aortic subregion by some hematopoi-etic, endothelial, and mesenchymal cells. In vivo analyses of IL-1RI - deficient embryos show an increased myeloid differentiation, concomitant with a slight decrease in AGM HSC activity. Our results suggest that IL-1 is an important homeostatic regulator at the earliest time of HSC development, acting to limit the differentiation of some HSCs along the myeloid lineage.

Published

2008

30. Analysis and manipulation of hematopoietic progenitor and stem cells from murine embryonic tissues

Author

Medvinsky, A. (Alexander), Taoudi, S. (Samir), Mendes, S.C. (Sandra), Dzierzak, E.A. (Elaine), Medvinsky, A. (Alexander), Taoudi, S. (Samir), Mendes, S.C. (Sandra), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic development begins in several locations in the mammalian embryo: yolk sac, aorta-gonad-mesonephros region (AGM), and the chorio-allantoic placenta. Generation of the most potent cells, adult definitive hematopoietic stem cells (HSCs), occurs within the body of the mouse embryo at midgestation in the AGM region. Similarly, at the equivalent developmental time in the human embryo, the AGM region has been shown to contain multipotent progenitors. Hence, the mouse embryo serves as an excellent model to study hematopoietic development. To further studies on the ontogeny of the adult hematopoietic system, the focus of this unit is on the experimental methods used in analysis of the AGM region.

Published

2008

31. The role of apoptosis in the development of AGM hematopoietic stem cells revealed by Bcl-2 overexpression

Author

Orelio, C., Harvey, K.N., Miles, C.G. (Colin), Oostendorp, R.A. (Robert), Horn, K. van der, Dzierzak, E.A. (Elaine), Orelio, C., Harvey, K.N., Miles, C.G. (Colin), Oostendorp, R.A. (Robert), Horn, K. van der, and Dzierzak, E.A. (Elaine)

Abstract

Apoptosis is an essential process in embryonic tissue remodeling and adult tissue homeostasis. Within the adult hematopoietic system, it allows for tight regulation of hematopoietic cell subsets. Previously, it was shown that B-cell leukemia 2 (Bcl-2) overexpression in the adult increases the viability and activity of hematopoietic cells under normal and/or stressful conditions. However, a role for apoptosis in the embryonic hematopoietic system has not yet been established. Since the first hematopoietic stem cells (HSCs) are generated within the aortagonad-mesonephros (AGM; an actively remodeling tissue) region beginning at embryonic day 10.5, we examined this tissue for expression of apoptosis-related genes and ongoing apoptosis. Here, we show expression of several proapoptotic and antiapoptotic genes in the AGM. We also generated transgenic mice overexpressing Bcl-2 under the control of the transcriptional regulatory elements of the HSC marker stem cell antigen-1 (Sca-1), to test for the role of cell survival in the regulation of AGM HSCs. We provide evidence for increased numbers and viability of Sca-1(+) cells in the AGM and subdissected midgestation aortas, the site where HSCs are localized. Most important, our in vivo transplantation data show that Bcl-2 overexpression increases AGM and fetal liver HSC activity, strongly suggesting that apoptosis plays a role in HSC development.

Published

2004

32. Cell-cell contact and anatomical compatibility in stromal cell-mediated HSC support during development

Author

Harvey, K. (Kirsten), Dzierzak, E.A. (Elaine), Harvey, K. (Kirsten), and Dzierzak, E.A. (Elaine)

Abstract

Hematopoietic stem cells (HSCs) are able to generate the wide variety of blood cells found in the adult and are maintained in the bone marrow (BM) stromal microenvironment. In the aorta-gonads-mesonephros (AGM), which autonomously generates the first HSCs, the stromal microenvironment is largely uncharacterized. We have previously made an extensive panel of stromal clones from AGM subregions and have found that clones from the urogenital ridges (UG) provide the most potent support for adult BM HSCs. However, it is unknown to what extent the stroma from this developmentally and anatomically distinct microenvironment can support HSCs from other regions of the embryo, such as yolk sac. Moreover, it is unknown whether cell-cell contact is necessary in this microenvironment. Here, we show that the HSCs from the embryonic aorta are the most potently supported HSCs in UG stromal clone co-cultures and that contact is required for the maintenance and expansion of embryo-derived HSCs.

Published

2004

33. GATA-2 plays two functionally distinct roles during the ontogeny of hematopoietic stem cells

Author

Ling, K-W. (Kam-Wing), Ottersbach, K. (Katrin), Hamburg, J.P. (Jan Piet) van, Oziemlak, A. (Aneta), Tsai, F.Y. (Fong-Ying), Orkin, S.H. (Stuart), Ploemacher, R.E. (Robert), Hendriks, R.W. (Rudi), Dzierzak, E.A. (Elaine), Ling, K-W. (Kam-Wing), Ottersbach, K. (Katrin), Hamburg, J.P. (Jan Piet) van, Oziemlak, A. (Aneta), Tsai, F.Y. (Fong-Ying), Orkin, S.H. (Stuart), Ploemacher, R.E. (Robert), Hendriks, R.W. (Rudi), and Dzierzak, E.A. (Elaine)

Abstract

GATA-2 is an essential transcription factor in the hematopoietic system that is expressed in hematopoietic stem cells (HSCs) and progenitors. Complete deficiency of GATA-2 in the mouse leads to severe anemia and embryonic lethality. The role of GATA-2 and dosage effects of this transcription factor in HSC

Published

2004

34. Impaired hematopoiesis in mice lacking the transcription factor Sp3

Author

Loo, P.F. van, Bouwman, R.J.P. (Peter), Ling, K-W. (Kam-Wing), Middendorp, S., Suske, G., Grosveld, F.G. (Frank), Dzierzak, E.A. (Elaine), Philipsen, J.N.J. (Sjaak), Hendriks, R.W. (Rudi), Loo, P.F. van, Bouwman, R.J.P. (Peter), Ling, K-W. (Kam-Wing), Middendorp, S., Suske, G., Grosveld, F.G. (Frank), Dzierzak, E.A. (Elaine), Philipsen, J.N.J. (Sjaak), and Hendriks, R.W. (Rudi)

Abstract

As the zinc-finger transcription factor specificity protein 3 (Sp3) has been implicated in the regulation of many hematopoietic-specific genes, we analyzed the role of Sp3 in hematopoiesis. At embryonic day 18.5 (E18.5), Sp3-/- mice exhibit a partial arrest of T-cell development in the thymus and B-cell numbers are reduced in liver and spleen. However, pre-B-cell proliferation and differentiation into immunoglobulin M-positive (IgM+) B cells in vitro are not affected. At E14.5 and E16.5, Sp3-/- mice exhibit a significant delay in the appearance of definitive erythrocytes in the blood, paralleled by a defect in the progression of differentiation of definitive erythroid cells in vitro. Perinatal death of the null mutants precludes the analysis of adult hematopoiesis in Sp3-/- mice. We therefore investigated the ability of E12.5 Sp3-/- liver cells to contribute to the hematopoietic compartment in an in vivo transplantation assay. Sp3-/- cells were able to repopulate the B- and T-lymphoid compartment, albeit with reduced efficiency. In contrast, Sp3-/- cells showed no significant engraftment in the erythroid and myeloid lineages. Thus, the absence of Sp3 results in cell-autonomous hematopoietic defects, affecting in particular the erythroid and myeloid cell lineages.

Published

2003

35. The Ly-6A (Sca-1) GFP transgene is expressed in all adult mouse hematopoietic stem cells

Author

Ma, X. (Xiaoqian), Robin, C.I., Ottersbach, K. (Katrin), Dzierzak, E.A. (Elaine), Ma, X. (Xiaoqian), Robin, C.I., Ottersbach, K. (Katrin), and Dzierzak, E.A. (Elaine)

Abstract

The Sca-1 cell surface glycoprotein is used routinely as a marker of adult hematopoietic stem cells (HSCs), allowing a >100-fold enrichment of these rare cells from the bone marrow of the adult mouse. The Sca-1 protein is encoded by the Ly-6A/E gene, a small 4-exon gene that is tightly controlled in its expression in HSCs and several hematopoietic cell types. For the ability to sort and localize HSCs directly from the mouse, we initiated a transgenic approach in which we created Ly-6A (Sca-1) green fluorescent protein (GFP) transgenic mice. We show here that a 14-kb Ly-6A expression cassette directs the transcription of the GFP marker gene in all functional repopulating HSCs in the adult bone marrow. A >100-fold enrichment of HSCs occurred by sorting for the GFP-expressing cells. Furthermore, as shown by fluorescence-activated cell sorting and histologic analysis of several hematopoietic tissues, the GFP transgene expression pattern generally corresponded to that of Sca-1. Thus, the Ly-6A GFP transgene facilitates the enrichment of HSCs and presents the likelihood of identifying HSCs in situ.

Published

2002

36. Embryonal subregion-derived stromal cell lines from novel temperature-sensitive SV40 T antigen transgenic mice support hematopoiesis

Author

Oostendorp, R.A. (Robert), Dzierzak, E.A. (Elaine), Medvinsky, A.J., Kusadasi, N. (Nuray), Nakayama, N., Harvey, K. (Kirsten), Orelio, C., Ottersbach, K. (Katrin), Covey, T., Ploemacher, R.E. (Robert), Saris, C. (Chris), Oostendorp, R.A. (Robert), Dzierzak, E.A. (Elaine), Medvinsky, A.J., Kusadasi, N. (Nuray), Nakayama, N., Harvey, K. (Kirsten), Orelio, C., Ottersbach, K. (Katrin), Covey, T., Ploemacher, R.E. (Robert), and Saris, C. (Chris)

Abstract

Throughout life, the hematopoietic system requires a supportive microenvironment that allows for the maintenance and differentiation of hematopoietic stem cells (HSC). To understand the cellular interactions and molecules that provide these functions, investigators have previously established stromal cell lines from the late gestational stage and adult murine hematopoietic microenvironments. However, the stromal cell microenvironment that supports the emergence, expansion and maintenance of HSCs during mid-gestational stages has been largely unexplored. Since several tissues within the mouse embryo are known to harbor HSCs (i.e. aortagonads-mesonephros, yolk sac, liver), we generated numerous stromal cell clones from these mid-gestational sites. Owing to the limited cell numbers, isolations were performed with tissues from transgenic embryos containing the ts SV40 Tag gene (tsA58) under the transcriptional control of constitutive and ubiquitously expressing promoters. We report here that the growth and cloning efficiency of embryonic cells (with the exception of the aorta) is increased in the presence of the tsA58 transgene. Furthermore, our results show that the large panel of stromal clones isolated from the different embryonal subregions exhibit heterogeneity in their ability to promote murine and human hematopoietic differentiation. Despite our findings of heterogeneity in hematopoietic growth factor gene expression profiles, high-level expression of some factors may influence hematopoietic differentiation. Interestingly, a few of these stromal clones express a recently described chordin-like protein, which is an inhibitor of bone morphogenic proteins and is preferentially expressed in cells of the mesenchymal lineage.

Published

2002

37. Definitive hematopoietic stem cells first develop within the major arterial regions of the mouse embryo.

Author

Bruijn, M.F.T.R. (Marella) de, Speck, N.A., Peeters, M.C. (Marian), Dzierzak, E.A. (Elaine), Bruijn, M.F.T.R. (Marella) de, Speck, N.A., Peeters, M.C. (Marian), and Dzierzak, E.A. (Elaine)

Abstract

The aorta-gonad-mesonephros (AGM) region is a potent hematopoietic site within the mammalian embryo body, and the first place from which hematopoietic stem cells (HSCs) emerge. Within the complex embryonic vascular, excretory and reproductive tissues of the AGM region, the precise location of HSC development is unknown. To determine where HSCs develop, we subdissected the AGM into aorta and urogenital ridge segments and transplanted the cells into irradiated adult recipients. We demonstrate that HSCs first appear in the dorsal aorta area. Furthermore, we show that vitelline and umbilical arteries contain high frequencies of HSCs coincident with HSC appearance in the AGM. While later in development and after organ explant culture we find HSCs in the urogenital ridges, our results strongly suggest that the major arteries of the embryo are the most important sites from which definitive HSCs first emerge.

Published

2000

38. CFU-S(11) activity does not localize solely with the aorta in the aorta-gonad-mesonephros region

Author

Bruijn, M.F.T.R. (Marella) de, Peeters, M.C. (Marian), Luteijn, T., Visser, P. (Pim), Speck, N.A., Dzierzak, E.A. (Elaine), Bruijn, M.F.T.R. (Marella) de, Peeters, M.C. (Marian), Luteijn, T., Visser, P. (Pim), Speck, N.A., and Dzierzak, E.A. (Elaine)

Abstract

The aorta-gonad-mesonephros (AGM) region is a potent hematopoietic site in the midgestation mouse conceptus and first contains colony-forming units-spleen day 11 (CFU-S(11)) at embryonic day 10 (E10). Because CFU-S(11) activity is present in the AGM region before the onset of hematopoietic stem cell (HSC) activity, CFU-S(11) activity in the complex developing vascular and urogenital regions of the AGM was localized. From E10 onward, CFU-S(11) activity is associated with the aortic vasculature, and is found also in the urogenital ridges (UGRs). Together with data obtained from organ explant cultures, in which up to a 16-fold increase in CFU-S(11) activity was observed, it was determined that CFU-S(11) can be increased autonomously both in vascular sites and in UGRs. Furthermore, CFU-S(11) activity is present in vitelline and umbilical vessels. This, together with the presence of CFU-S(11) in the UGRs 2 days before HSC activity, suggests both temporally and spatially distinct emergent sources of CFU-S(11). (Blood. 2000;96:2902-2904)

Published

2000

39. Embryonic beginnings of definitive hematopoietic stem cells

Author

Dzierzak, E.A. (Elaine) and Dzierzak, E.A. (Elaine)

Published

1999

40. Definitive hematopoiesis is autonomously initiated by the AGM region

Author

Medvinsky, A. (Alexander), Dzierzak, E.A. (Elaine), Medvinsky, A. (Alexander), and Dzierzak, E.A. (Elaine)

Published

1996

41. Development of hematopoietic stem cell activity in the mouse embryo.

Author

Müller, A.M. (Albrecht), Medvinsky, A., Strouboulis, J. (John), Grosveld, F.G. (Frank), Dzierzak, E.A. (Elaine), Müller, A.M. (Albrecht), Medvinsky, A., Strouboulis, J. (John), Grosveld, F.G. (Frank), and Dzierzak, E.A. (Elaine)

Abstract

The precise time of appearance of the first hematopoietic stem cell activity in the developing mouse embryo is unknown. Recently the aorta-gonad-mesonephros region of the developing mouse embryo has been shown to possess hematopoietic colony-forming activity (CFU-S) in irradiated recipient mice. To determine whether the mouse embryo possesses definitive hematopoietic stem cell activity in the analogous AGM region and to determine the order of appearance of stem cells in the yolk sac, AGM region, and liver, we transferred these embryonic tissues into adult irradiated recipients. We report here the long-term, complete, and functional hematopoietic repopulation of primary and serial recipients with AGM-derived cells. We observe potent hematopoietic stem cell activity in the AGM region before the appearance of yolk sac and liver stem cell activity and discuss a model for the maturation of stem cell activity in mouse embryogenesis.

Published

1994