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Prepublished online as a Blood First Edition Paper on November 7, 2002; DOI 10.1182/blood-2002-05-1477.
RED CELLS
From the Department of Hematology and Oncology,
Istituto Superiore di Sanità, Rome, Italy; and the
Kimmel Cancer Center, Thomas Jefferson University, Philadelphia, PA.
Mechanisms underlying fetal hemoglobin (HbF) reactivation in stress
erythropoiesis have not been fully elucidated. We suggested that a key
role is played by kit ligand (KL). Because glucocorticoids (GCs)
mediate stress erythropoiesis, we explored their capacity to potentiate
the stimulatory effect of KL on HbF reactivation, as evaluated in
unilineage erythropoietic culture of purified adult progenitors
(erythroid burst-forming units [BFU-Es]). The GC derivative
dexamethasone (Dex) was tested in minibulk cultures at graded dosages
within the therapeutical range (10 Human hemoglobin (Hb) is heterogeneous at all
stages of development, from embryonic through adult life. The fetal
period is characterized by the synthesis of fetal Hb (HbF, Cell cultures and animal models have allowed the identification of
several agents reactivating HbF synthesis,9 including chemical inducers and cytokines. The clinical use of hydroxyurea, though partially successful in the treatment of sickle cell
anemia,10,11 has been hindered by myelotoxicity, potential
long-term carcinogenicity, and only moderate therapeutic effects in
most patients.12 Histone deacetylase inhibitors,
particularly butyrate analogs, increase HbF levels in primary cultures
of human erythroid cells.13 Their clinical use, however,
is rendered difficult by their rapid degradation. In sickle cell
anemia, the intravenous administration of arginine butyrate enhances
HbF synthesis, but the effect gradually declines on prolonged infusion.
Pulse regimens may offset this decline but may result in a suboptimal
amount of the drug and a lower stimulatory effect.14
In addition to chemical inducers, HbF synthesis may be stimulated by
hematopoietic growth factors (HGFs).15-18 Particularly, kit ligand (KL) markedly stimulated HbF production in sickle cell anemia17 and healthy hematopoietic progenitor cell (HPC)
cultures.18 In vitro, the stimulating effect of KL is
potentiated by histone deacetylase inhibitors; however, these chemical
inducers, particularly when used alone, exert an inhibitory effect on
erythropoiesis.19 In vivo KL stimulates HbF synthesis and
potentiates the effects of hydroxyurea.20 Here again, the
combined administration of KL and hydroxyurea in the clinical setting
is limited by the toxic effects of the latter agent.
To overcome these limitations, we have explored whether the stimulating
effect of KL may be potentiated by other therapeutic agents widely used
in the clinical setting. Among the hormones that stimulate
erythropoiesis, glucocorticoids (GCs) are of particular interest, as
indicated by in vitro and in vivo studies.21-23 We have
therefore investigated the effects of the GC derivative dexamethasone (Dex) on HbF reactivation in erythroid bursts generated by purified adult erythroid burst-forming units (BFU-Es) in minibulk and
single-cell unilineage erythroid cultures. The results indicate that
Dex alone does not affect HbF reactivation and erythroid cell
proliferation, whereas combined treatment with Dex and KL exerts a
synergistic stimulatory effect on both parameters.
Recombinant human HGFs and chemical inducers
HPC purification
The CD34+ HPCs were then purified by using the MiniMACS CD34 isolation system (Miltenyi, Bergisch Gladbach, Germany) following the manufacturer's instructions. Purified cells were more than 90% CD34+, as evaluated by fluorescence-activated cell sorting (FACS) analysis. HPC unilineage erythropoietic culture Mini-bulk culture.
Purified HPCs were grown in fetal calf serum (FCS)-free liquid culture
(5 × 104 cells/mL/well) in a fully humidified atmosphere
of 5% CO2/5% O2/90% N2 and were
induced to unilineage erythropoietic differentiation by an
erythroid-specific HGF cocktail (EPO and low-dose IL-3/GM-CSF), as
reported.25,26 The HGF cocktail was supplemented or not supplemented with KL (100 ng/mL), Dex (10 Unicellular sibling BFU-E culture.
Unicellular cultures (0.5 cell/well) were performed in flat-bottomed
96-microwell plates in 0.1 mL FCS-free medium25-27
supplemented with 5% FCS. To selectively stimulate erythroid
differentiation, the cultures were supplemented with the HGF cocktail
(EPO and IL-3/GM-CSF) indicated in the previous paragraph. At
days 3 to 4, the 4 cell clones were identified. The 4 sibling cells
picked up by a micromanipulator were seeded in 4 different
wells,19 each containing 0.1 mL of the same erythroid
medium supplemented with plateau levels of KL (100 ng/mL), alone or
combined with graded amounts of Dex
(10 Morphology analysis. Cells were harvested from day 14 through day 28, smeared on glass slides by cytospin centrifugation, and stained with standard May-Grünwald-Giemsa. For single sibling colony analysis, polylysine-coated glass slides were used. HbF assays: F-cell number and F cells The percentage of mature erythroblasts containing HbF was evaluated by indirect fluorescence as previously described.3 Briefly, erythroid cells were cytocentrifuged on a glass slide, fixed for 5 minutes in acetone-methanol (9:1, vol/vol), washed 3 times with phosphate-buffered saline (PBS) and once with PBS containing 2 mg/mL bovine serum albumin (BSA), and incubated for 40 minutes at 37°C with anti-human HbF monoclonal antibody (mAb; Caltag Laboratories, Burlingame, CA). Slides were washed twice with PBS and once with PBS/BSA, incubated for 30 minutes at room temperature with fluorescein isothiocyanate (FITC)-conjugated F(ab')2 antimouse immunoglobulin G (IgG; Dakopatts, Copenhagen, Denmark), and extensively washed in PBS. Slides were then mounted in PBS/glycerol (50:50) and observed under an Axiophot Zeiss microscope (Zeiss, Jena, Germany) equipped for fluorescence. As a negative control, cells were incubated with healthy mouse IgG instead of anti-HbF and were processed as indicated above in this paragraph.In some experiments, HbF containing erythroblasts were also evaluated by flow cytometry. Briefly, erythroid cells were fixed and permeabilized with the Cytofix/Cytoperm kit (PharMingen, San Diego, CA), washed in PBS containing 0.1% Triton X-100, incubated with anti-HbF mAb, and then washed with anti-mouse IgG antibody, as indicated above. The percentage of fluorescent cells and the intensity of fluorescence (mean fluorescence intensity [MFI]) were evaluated using a FACScan (Becton Dickinson, San Diego, CA).
Id2, Tal1, and GATA1 expression Id2, Tal1, and GATA1 expression was investigated at the protein level by Western blotting on erythroid minibulk cultures. Briefly, 2.5 × 105 cells were obtained at different days of erythroid culture and were lysed in 20 µL boiling sodium dodecyl sulfate (SDS) sample buffer. Samples were boiled for 10 minutes and then centrifuged at 10 000 rpm for 10 minutes at 4°C to remove debris. Whole cell lysates were resolved by SDS-polyacrylamide gel electrophoresis. The same lysate amount was added to all lanes. Tal1, Id2, and GATA1 expression were detected using an anti-Tal1 rabbit serum 1080,29 an anti-Id2 rabbit polyclonal antibody sc-489, and an anti- GATA1 rat monoclonal antibody sc-266 (Santa Cruz Biotechnology, CA), respectively. Anti- actin CP01 (Oncogene,
Boston, MA) was used as loading control.
In the first series of experiments we analyzed the effect of Dex
in minibulk erythroid culture. This synthetic glucocorticoid was added
in a dose-response fashion (10 When used in combination with KL, Dex at the 10
Evaluation of F-cell frequency by immunofluorescence (IF) in minibulk
erythroid cultures showed that Dex alone slightly reactivated the
production of F erythroblasts (from 4% in control erythroid cultures
to 12% at 10
This striking HbF reactivation was confirmed by analysis of
In a second series of experiments we analyzed the effects of Dex, alone
or in combination with KL, in sibling BFU-E colonies. Briefly, the
purified HPCs were grown in unicellular unilineage erythroid liquid
cultures. After 2 cell divisions, the 4 sibling BFU-Es were subdivided
by micromanipulation and individually reseeded in secondary erythroid
cultures supplemented with KL ± Dex from 10
Id2 protein was clearly detected in quiescent HPCs and in all culture
conditions during the first 2 days of culture. Starting from day 2, the
expression decreased in control (C) and Dex cultures and
slightly increased in KL and KL + Dex cultures. From day 4 of
culture to terminal maturation, Id2 protein was virtually undetectable in control erythroid cultures supplemented or not supplemented with
Dex. In contrast, it was expressed at sustained levels up to day 18 and
day 26 in KL and KL + Dex cultures, respectively (Figure
5A). Specifically, Id2 expression
remained detectable to day 26 only in KL cultures supplemented with Dex
ranging from 10
As shown in Figure 5A, Tal1 protein was virtually undetectable in
quiescent HPCs. In control cultures, supplemented or not with Dex
10 GATA1 expression, virtually undetectable in quiescent HPCs and until day 2 of culture, was induced at day 4 in all erythroid cultures, supplemented or not with KL and Dex (Figure 5A). In control ± Dex wells, GATA1 protein was detectable to day 14, whereas in KL and KL + Dex cultures, GATA1 was extended to day 21 and day 26, respectively (Figure 5A).
Stress erythropoiesis is triggered by tissue hypoxia, which may be induced by blood loss, anemia, or oxygen deprivation. It has been established that GCs are important mediators of erythropoietic stress. GCs regulate a variety of physiological responses and developmental processes by binding to their cognate nuclear receptor GCR.30,31 In vitro, the GCR cooperates with the activated EPO receptor (EPOR) and Kit to induce long-term proliferation of erythroid progenitors while delaying their differentiation.22 In vivo, GCR is also required for the rapid expansion of murine erythroid progenitors under stress conditions such as erythrolysis or hypoxia.23 In postnatal conditions associated with erythropoietic stress, HbF
synthesis is reactivated up to 10% to 20% relative Here again, we observed a direct correlation between the enhanced erythroid proliferation and the reactivation of HbF, as previously reported18,19 and confirmed by others.34 We suggest that in adult stress erythropoiesis, HbF synthesis may be reactivated by enhanced proliferation of early erythroid cells, triggered by KL and GCs. Hypothetically, a decline of KL activity may similarly mediate perinatal Hb switching. Indeed, erythroid cell proliferation is elevated in fetal life, gradually declines in the perinatal period, and bottoms in steady-state adult life.35 KL activity is more elevated in fetal/perinatal life than in postnatal life, including the erythropoietic response to KL.36,37 Ongoing studies aim to verify this model of Hb switching. The effects of GCs on erythropoiesis have been investigated in cultures
stimulated by EPO only or by EPO and KL. In erythroid cultures of
unpurified fetal liver HPCs stimulated with EPO alone, Dex exerts a
dose-dependent inhibitory effect.38 This report is in line
with our observations on purified adult HPCs in control erythroid
cultures that show a dose-related inhibitory effect at
10 To shed light on the molecular mechanisms underlying the stimulatory
effects of KL + Dex on erythroid cell proliferation and HbF
synthesis, we have analyzed the expression of Id2, Tal1, and GATA1
transcription factors (TFs) at the protein level in erythroid cultures.
Circumstantial evidence suggests that Id2 and Tal1 may stimulate HbF
production. Specifically, Id2 enhances We observed that Id2 protein, though expressed in CD34+ cells, is gradually suppressed in control ± Dex cultures at days 1 to 2, down to undetectable levels from day 4. In sharp contrast, Id2 expression is sustained in the KL culture, particularly if supplemented with Dex, suggesting that Id2 may significantly contribute to stimulate erythroid cell proliferation and to delay erythroblast maturation. Because enhanced erythroid proliferation strictly correlates with and possibly causes HbF reactivation,18,19,34 it is hypothesized that the persistent Id2 expression induced by the addition of KL ± Dex may stimulate early erythroid proliferation and hence HbF synthesis. Our observations are in line with other reports on the proliferative and antidifferentiative Id2 effects in diverse hematopoietic cell types.43 Specifically, Id2-deficient mice show defective natural killer (NK) cell differentiation and lymph node formation.44,45 Furthermore, Id2 exerts a negative role in erythroid29 and B-lymphoid46 differentiation. In both lineages Id2 is expressed in early precursors but not in mature cells.29,47 Our observations on erythroid cell differentiation here and in our earlier report29 are apparently at variance with studies by Zhang et al,47 which report Id2 expression in maturing erythroid precursors. This discrepancy may be reconciled in view of the sharp differences in cell culture conditions (unpurified vs purified hemopoietic progenitor cells, serum-rich vs serum-free medium). Tal1 and GATA1, though undetectable in HPCs, are induced in erythroid culture. Specifically, Tal1 is detected in KL ± Dex cultures26,29 starting from day 1; interestingly, the induction in control ± Dex wells starts on day 2 and is altogether less pronounced in the initial culture period. In all groups, GATA1 is induced from day 4 onward. In all culture conditions, the expression of both TFs is sustained and declines in terminal erythroid cells. Therefore, the expression is more prolonged with KL ± Dex addition (as reported by Miller et al48 for Tal1), which induces a more extensive erythroid proliferation period. The initial enhancement of Tal1 expression induced by KL ± Dex may contribute to stimulate early erythroid proliferation. Indeed, Tal1 potentiates antiapoptotic mechanisms in early erythropoiesis (R. De Maria et al, manuscript submitted). On the other hand, Tal1 enhances c-kit expression and thereby maintains the sensitivity of erythroid cells to KL.49 Along these lines, the KL-induced prolongation of GATA1 expression may contribute to potentiate erythroblast proliferation. To clarify the molecular mechanisms underlying HbF reactivation, studies on transduction of Id2, Tal1, and GATA1 genes are in progress and will be presented in a separate report. It is noteworthy that the peak effect of Dex on erythroid cell
proliferation and HbF reactivation was observed at 10
We thank M. Blasi and M. Fontana for editorial assistance and A. Zito for the graphics.
Submitted May 23, 2002; accepted October 8, 2002.
Prepublished online as Blood First Edition Paper, November 7, 2002; DOI 10.1182/blood-2002-05-1477.
Supported in part by an intramural grant from the Istituto Superiore di Sanitá, Rome, Italy (M.G.).
M.G. and U.T. contributed equally to this manuscript.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Cesare Peschle, Kimmel Cancer Center, Room 609, Thomas Jefferson University, 233 South 10th St, Philadelphia, PA 19107-5541; e-mail: cesare.peschle{at}mail.tju.edu.
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  L. M. Starnes, A. Sorrentino, E. Pelosi, M. Ballarino, O. Morsilli, M. Biffoni, S. Santoro, N. Felli, G. Castelli, M. L. De Marchis, et al. NFI-A directs the fate of hematopoietic progenitors to the erythroid or granulocytic lineage and controls {beta}-globin and G-CSF receptor expression Blood, August 27, 2009; 114(9): 1753 - 1763. [Abstract] [Full Text] [PDF]
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M. Gabbianelli, O. Morsilli, A. Massa, L. Pasquini, P. Cianciulli, U. Testa, and C. Peschle Effective erythropoiesis and HbF reactivation induced by kit ligand in -thalassemia Blood, January 1, 2008; 111(1): 421 - 429. [Abstract] [Full Text] [PDF]
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B. L. Ebert, M. M. Lee, J. L. Pretz, A. Subramanian, R. Mak, T. R. Golub, and C. A. Sieff An RNA interference model of RPS19 deficiency in Diamond-Blackfan anemia recapitulates defective hematopoiesis and rescue by dexamethasone: identification of dexamethasone-responsive genes by microarray Blood, June 15, 2005; 105(12): 4620 - 4626. [Abstract] [Full Text] [PDF]
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Top
Abstract
Introduction
6 to 10
-globin content at terminal maturation (ie, in more
than 80%-90% mature erythroblasts). Equivalent results were obtained
in unicellular erythroid cultures of sibling BFU-Es treated with KL
alone or combined with graded amounts of Dex. These results indicate
that the stimulatory effect of KL + Dex is related to the
modulation of 
2 
HbA perinatal switch. More important,
therapeutic administration of agents stimulating HbF production may be
beneficial in patients with 
