MtDNA mutagenesis impairs elimination of mitochondria during erythroid maturation leading to enhanced erythrocyte destruction

K.J. Ahlqvist; S. Leoncini; A. Pecorelli; S.B. Wortmann; S. Ahola; S. Forsström; R. Guerranti; C. De Felice; J. Smeitink; L. Ciccoli; R.H. Hämäläinen; A. Suomalainen

doi:10.1038/ncomms7494

Erythrocyte Destruction by Prosthetic Heart Valves

Circulation ◽

10.1161/01.cir.37.4s2.ii-86 ◽

1968 ◽

Vol 37 (4s2) ◽

Cited By ~ 8

Author(s):

ROBERT A. INDEGLIA ◽

MICHAEL A. SHEA ◽

RICHARD L. VARCO ◽

EUGENE F. BERNSTEIN

Keyword(s):

Heart Valves ◽

Prosthetic Heart Valves ◽

Erythrocyte Destruction

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Genetic manipulation of RPS5 gene expression modulates the initiation of commitment of MEL cells to erythroid maturation: Implications in understanding ribosomopathies

International Journal of Oncology ◽

10.3892/ijo.2015.3017 ◽

2015 ◽

Vol 47 (1) ◽

pp. 303-314 ◽

Cited By ~ 3

Author(s):

IOANNIS S. VIZIRIANAKIS ◽

ELENI T. PAPACHRISTOU ◽

PANAGIOTIS ANDREADIS ◽

ELENA ZOPOUNIDOU ◽

CHRISTINA N. MATRAGKOU ◽

...

Keyword(s):

Gene Expression ◽

Genetic Manipulation ◽

Erythroid Maturation

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Chicken fetal antigen expression on the definitive erythroid maturation series in the bone marrow of the adult chicken

Journal of Experimental Zoology ◽

10.1002/jez.1402120113 ◽

1980 ◽

Vol 212 (1) ◽

pp. 101-108 ◽

Cited By ~ 10

Author(s):

Carrie H. Nelson ◽

Nipam H. Patel ◽

Bob G. Sanders

Keyword(s):

Bone Marrow ◽

Antigen Expression ◽

Adult Chicken ◽

Erythroid Maturation ◽

Fetal Antigen

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Erythroid-cell-specific properties of transcription factor GATA-1 revealed by phenotypic rescue of a gene-targeted cell line.

Molecular and Cellular Biology ◽

10.1128/mcb.17.3.1642 ◽

1997 ◽

Vol 17 (3) ◽

pp. 1642-1651 ◽

Cited By ~ 240

Author(s):

M J Weiss ◽

C Yu ◽

S H Orkin

Keyword(s):

Transcription Factor ◽

Cell Line ◽

Zinc Finger ◽

Es Cells ◽

Embryonic Stem ◽

Erythroid Cell ◽

Transactivation Domain ◽

Stage Of Development ◽

Erythroid Maturation

The zinc finger transcription factor GATA-1 is essential for erythropoiesis. In its absence, committed erythroid precursors arrest at the proerythroblast stage of development and undergo apoptosis. To study the function of GATA-1 in an erythroid cell environment, we generated an erythroid cell line from in vitro-differentiated GATA-1- murine embryonic stem (ES) cells. These cells, termed G1E for GATA-1- erythroid, proliferate as immature erythroblasts yet complete differentiation upon restoration of GATA-1 function. We used rescue of terminal erythroid maturation in G1E cells as a stringent cellular assay system in which to evaluate the functional relevance of domains of GATA-1 previously characterized in nonhematopoietic cells. At least two major differences were established between domains required in G1E cells and those required in nonhematopoietic cells. First, an obligatory transactivation domain defined in conventional nonhematopoietic cell transfection assays is dispensable for terminal erythroid maturation. Second, the amino (N) zinc finger, which is nonessential for binding to the vast majority of GATA DNA motifs, is strictly required for GATA-1-mediated erythroid differentiation. Our data lead us to propose a model in which a nuclear cofactor(s) interacting with the N-finger facilitates transcriptional action by GATA-1 in erythroid cells. More generally, our experimental approach highlights critical differences in the action of cell-specific transcription proteins in different cellular environments and the power of cell lines derived from genetically modified ES cells to elucidate gene function.

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Resveratrol accelerates erythroid maturation by activation of FoxO3 and ameliorates anemia in beta-thalassemic mice

Haematologica ◽

10.3324/haematol.2013.090076 ◽

2013 ◽

Vol 99 (2) ◽

pp. 267-275 ◽

Cited By ~ 58

Author(s):

S. S. Franco ◽

L. De Falco ◽

S. Ghaffari ◽

C. Brugnara ◽

D. A. Sinclair ◽

...

Keyword(s):

Erythroid Maturation

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Hypoxic stress underlies defects in erythroblast islands in the Rb-null mouse

Blood ◽

10.1182/blood-2007-01-069104 ◽

2007 ◽

Vol 110 (6) ◽

pp. 2173-2181 ◽

Cited By ~ 19

Author(s):

Benjamin T. Spike ◽

Benjamin C. Dibling ◽

Kay F. Macleod

Keyword(s):

Fetal Liver ◽

Cell Maturation ◽

Null Mouse ◽

Hypoxic Stress ◽

Red Cell ◽

Exogenous Stress ◽

Erythroid Maturation ◽

Definitive Erythropoiesis

Abstract Definitive erythropoiesis occurs in islands composed of a central macrophage in contact with differentiating erythroblasts. Erythroid maturation including enucleation can also occur in the absence of macrophages both in vivo and in vitro. We reported previously that loss of Rb induces cell-autonomous defects in red cell maturation under stress conditions, while other reports have suggested that the failure of Rb-null erythroblasts to enucleate is due to defects in associated macrophages. Here we show that erythropoietic islands are disrupted by hypoxic stress, such as occurs in the Rb-null fetal liver, that Rb−/− macrophages are competent for erythropoietic island formation in the absence of exogenous stress and that enucleation defects persist in Rb-null erythroblasts irrespective of macrophage function.

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Hematopoietic-Specific CSNK2B Loss in Mice Causes Impaired Erythropoiesis

Blood ◽

10.1182/blood.v130.suppl_1.82.82 ◽

2017 ◽

Vol 130 (Suppl_1) ◽

pp. 82-82

Author(s):

Laura Quotti Tubi ◽

Sara Canovas Nunes ◽

Marilena Carrino ◽

Ketty Gianesin ◽

Sabrina Manni ◽

...

Keyword(s):

Western Blot ◽

Cell Viability ◽

Knockout Mice ◽

Cell Biology ◽

Combined Treatment ◽

Conditional Knockout ◽

Erythroid Cell ◽

Red Cell ◽

Erythroid Cells ◽

Erythroid Maturation

Abstract CK2 (Csnk2, casein kinase 2) is a Ser-Thr kinase composed by two catalytic (α) and two regulatory (β) subunits and involved in the regulation of various signaling cascades, which are critical for stem cell biology and hematopoietic development. However, a direct role for CK2 during blood cell differentiation is still undefined. Here, we examined the function of CK2 in erythropoiesis by using a hematopoietic-specific conditional knockout mouse model of the β regulatory subunit (Vav1-CRE x Csnk2β f/f mice). Since CK2β knockout mice died in utero, the study was carried out during gestation collecting fetuses from 12.5 to 17.5 days post conception (dpc) and performing the analysis on fetal liver. CK2β knockout fetuses were pale and hydropic, displayed a smaller liver, disarrayed vascularization and haemorrhages. Lack of CK2β caused depletion of hematopoietic/precursor cells, in particular of common lymphoid progenitors and megakaryocyte-erythrocyte progenitors. CK2β loss resulted to affect both early and late erythroid maturation and red cell viability. CK2β knockout contained lower numbers of TER119 positive cells, which displayed a down modulation of the surface expression of transferrin receptor (CD71) and an increased spontaneous apoptosis. Erythroid cells showed alterations in morphology compatible with myelodysplastic changes. Loss of CK2β caused alterations of erythroid cell proliferation, which was different depending on the stage of erythroid maturation: indeed, BrdU and 7AAD staining showed that less mature erythroid cells (CD71+Ter119-) had a lower rate of proliferation but a normal viability; on the contrary, more mature (CD71-Ter119+) erythroid cells suffered in part of apoptosis and in part accumulated in the S phase. RNA seq analysis performed on purified Ter119+ cells revealed upregulation of TP53 -associated genes as well as of Cdkn1a (p21); on the contrary, there was a down-modulation of Stat5 (an erythropoietin receptor down-stream effector) and genes involved in red cell survival and differentiation in particular c-kit and genes associated to the PI3/Akt pathway. The expression of adhesion molecules and surface carriers for inorganic cations/anionsimportant for the osmotic equilibrium and cell membrane integrity was also found markedly dysregulated. Real time quantitative PCR and Western Blot (WB) analyses confirmed the expression data of Cdkn1a, c-Kit, Bcl-xL, Jak-Stat5 as well as of Akt-Gata-1 axis. Gata-1, the key transcription factor for definitive erythropoiesis, was reduced in CK2β knockout mice as were its downstream target genes such as Alas-2, Lrf, Eklf, Epo-R, β-globin. Immature fetal globins accumulated. In order to find a molecular mechanism, we used an in vitro model of erythroid differentiation based on G1ER cells, an estrogen inducible GATA-1 null murine erythroblast cell line; the combined treatment of β-estradiol and inhibition of CK2 through the chemical inhibitor CX-4945 or RNA interference against CK2β confirmed the negative effect on differentiation. Western blot analysis indicated a potential role of the kinase in the regulation of Akt, Gata-1 and Stat5 protein stability. Moreover, the blockade or down modulation of CK2 caused changes in Gata-1 nuclear distribution with loss of the speckled pattern induced by β-estradiol. Thus, CK2 is a likely essential controller of GATA-1 transcriptional function. Altogether, our work demonstrates that CK2 is a master regulator of erythroid development, by impinging on Stat5, Akt and Gata-1 signaling and influencing red cell viability, bioenergetics, proliferation and maturation. Disclosures No relevant conflicts of interest to declare.

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Chromatin Accessibility Mapping of Primary Erythroid Cell Populations Leads to Identification and Validation of Nuclear Factor I X (NFIX) As a Novel Fetal Hemoglobin (HbF) Repressor

Blood ◽

10.1182/blood-2019-124337 ◽

2019 ◽

Vol 134 (Supplement_1) ◽

pp. 812-812

Author(s):

Mudit Chaand ◽

Chris Fiore ◽

Brian T Johnston ◽

Diane H Moon ◽

John P Carulli ◽

...

Keyword(s):

Gene Expression ◽

Globin Gene ◽

Chromatin Accessibility ◽

Cell Populations ◽

Rna Seq ◽

Globin Mrna ◽

Employment Equity ◽

Equity Ownership ◽

Erythroid Maturation ◽

Globin Gene Expression

Human beta-like globin gene expression is developmentally regulated. Erythroblasts (EBs) derived from fetal tissues, such as umbilical cord blood (CB), primarily express gamma globin mRNA (HBG) and HbF, while EBs derived from adult tissues, such as bone marrow (BM), predominantly express beta globin mRNA (HBB) and adult hemoglobin. Human genetics has validated de-repression of HBG in adult EBs as a powerful therapeutic paradigm in diseases involving defective HBB, such as sickle cell anemia. To identify novel factors involved in the switch from HBG to HBB expression, and to better understand the global regulatory networks driving the fetal and adult cell states, we performed transcriptome profiling (RNA-seq) and chromatin accessibility profiling (ATAC-seq) on sorted EB cell populations from CB or BM. This approach improves upon previous studies that used unsorted cells (Huang J, Dev Cell 2016) or that did not measure chromatin accessibility (Yan H, Am J Hematol 2018). CD34+ cells from CB and BM were differentiated using a 3-phase in vitro culture system (Giarratana M, Blood 2011). Fluorescence-activated cell sorting and the cell surface markers CD36 and GYPA were used to isolate 7 discrete populations, with each sorting gate representing increasingly mature, stage-matched EBs from CB or BM (Fig 1A, B). RNA-seq analysis revealed expected expression patterns of the beta-like globins, with total levels increasing during erythroid maturation and primarily composed of HBB or HBG transcripts in BM or CB, respectively (Fig 1C). Erythroid maturation led to progressive increases in chromatin accessibility at the HBB promoter in BM populations. In CB-derived cells, erythroid maturation led to progressive increases in chromatin accessibility at the HBG promoters through the CD36+GYPA+ stage (Pops 1-5). Chromatin accessibility shifted from the HBG promoters to the HBB promoter during the final stages of differentiation (Pops 6-7), suggesting that HBG gene activation is transient in CB EBs (Fig 1D). Hierarchical clustering and principal component analysis of ATAC-seq data revealed that cell populations cluster based on differentiation stage rather than by BM or CB lineage, suggesting most molecular changes are stage-specific, not lineage-specific (Fig 2A, B). To identify transcription factors driving cell state, and potentially beta-like globin expression preference, we searched for DNA binding motifs within regions of differential chromatin accessibility and found NFI factor motifs enriched under peaks that were larger in BM relative to CB (Fig 2C). Transcription factor footprinting analysis showed that both flanking accessibility and footprint depth at NFI motifs were also increased in BM relative to CB (Fig 2D). Increased chromatin accessibility was observed at the NFIX promoter in BM relative to CB populations, and in HUDEP-2 relative to HUDEP-1 cell lines (Fig 2E). Furthermore, accessibility at the NFIX promoter correlated with elevated NFIX mRNA in BM and HUDEP-2 relative to CB and HUDEP-1, respectively. Together these data implicated NFIX in HbF repression, a finding consistent with previous genome-wide association and DNA methylation studies that suggested a possible role for NFIX in regulating beta-like globin gene expression (Fabrice D, Nat Genet 2016; Lessard S, Genome Med 2015). To directly test the hypothesis that NFIX represses HbF, short hairpin RNAs were used to knockdown (KD) NFIX in primary erythroblasts derived from human CD34+ BM cells (Fig 3A). NFIX KD led to a time-dependent induction of HBG mRNA, HbF, and F-cells comparable to KD of the known HbF repressor BCL11A (Fig 3B-D). A similar effect on HbF was observed in HUDEP-2 cells following NFIX KD (Fig 3E). Consistent with HbF induction, NFIX KD also increased chromatin accessibility and decreased DNA methylation at the HBG promoters in primary EBs (Fig 3F, G). NFIX KD led to a delay in erythroid differentiation as measured by CD36 and GYPA expression (Fig 3H). Despite this delay, by day 14 a high proportion of fully enucleated erythroblasts was observed, suggesting NFIX KD cells are capable of terminal differentiation (Fig 3H). Collectively, these data have enabled identification and validation of NFIX as a novel repressor of HbF, a finding that enhances the understanding of beta-like globin gene regulation and has potential implications in the development of therapeutics for sickle cell disease. Disclosures Chaand: Syros Pharmaceuticals: Employment, Equity Ownership. Fiore:Syros Pharmaceuticals: Employment, Equity Ownership. Johnston:Syros Pharmaceuticals: Employment, Equity Ownership. Moon:Syros Pharmaceuticals: Employment, Equity Ownership. Carulli:Syros Pharmaceuticals: Employment, Equity Ownership. Shearstone:Syros Pharmaceuticals: Employment, Equity Ownership.

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Immunophenotype of Erythroid Precursors in Patient with Pure Red Cell Aplasia (PRCA): Utility of Analysis of Erythroid Maturation

Annals of Hematology & Oncology ◽

10.26420/annhematoloncol.2021.1346 ◽

2021 ◽

Vol 8 (5) ◽

Author(s):

Jerez J ◽

◽

Ocqueteau M ◽

Keyword(s):

Correct Diagnosis ◽

Standard Of Care ◽

Pure Red Cell Aplasia ◽

Refractory Anemia ◽

Red Cell ◽

Red Cell Aplasia ◽

Bone Marrow Histology ◽

Erythroid Precursors ◽

Normochromic Anemia ◽

Erythroid Maturation

Pure Red Cell Aplasia (PRCA) is an infrequent disease [1,2], which usually presents as hypogenerative normochromic anemia, and is characterized by a significant decrease (including absence) of erythroid precursors [3]. Its etiology can be congenital or acquired, and its correct diagnosis requires exclusion of alternative cases of refractory anemia, so the bone marrow histology plays a crucial role. Myelodisplastic Syndromes (MDS) should always be considered in its differential diagnosis. The use of laboratory tools, specifically Flow Cytometry (FCM) is gained importance in the study of malignant and benign hematology pathologies. In MDS, FCM is not yet considered a standard of care, however it provides valuable information [4,5] and there are numerous publications and scores for its usual clinical use (for example Ogata score and RED-score [6,7]). In relation to the rise of FCM in MDS, enormous progress has been made in the description of the erythroid precursors immunophenotype [8-10]. An example of normal erythroid maturation is presented in Figure 1, showing proerythroblasts with immunophenotype CD71+ CD105+ CD117+, basophilic erythroblasts CD71+ CD105+ CD117-, polychromatophilic and orthochromatophilic erythroblasts CD71+ CD105- CD117- distinguishing by size in Forward Scatter (FSC) versus CD36 respectively. Characteristic maturation curve in CD117 versus CD105 analysis evidenced a predominance towards more mature erythroblasts.

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Coordinate glycosylation and cell surface expression of glycophorin A during normal human erythropoiesis

Blood ◽

10.1182/blood.v70.6.1959.bloodjournal7061959 ◽

1987 ◽

Vol 70 (6) ◽

pp. 1959-1961

Author(s):

MR Loken ◽

CI Civin ◽

WL Bigbee ◽

RG Langlois ◽

RH Jensen

Keyword(s):

Surface Expression ◽

Cell Surface Expression ◽

Glycophorin A ◽

Constant Amount ◽

Normal Human ◽

Erythroid Maturation ◽

Highly Correlated ◽

Erythroid Development ◽

Maximum Expression ◽

Normal Human Bone Marrow

The expression of two epitopes on glycophorin A (GPA) during erythroid development was examined on normal human bone marrow using quantitative flow cytometry. The highly correlated binding of two monoclonal antibodies, one sensitive and the other insensitive to glycosylation, indicated that the two epitopes were coordinately expressed during erythroid development. Both antigens reached a maximum expression during the early normoblast stage and were maintained at a constant amount per cell throughout further maturation to erythrocytes. These data suggest that glycosylation of GPA, as detected by antibodies recognizing blood group (M) and (N) antigens, does not increase during erythroid maturation.

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