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Blood, Vol. 95 No. 12 (June 15), 2000:
pp. 3758-3764
HEMATOPOIESIS
From the FR 60, Biologie des Greffes, Université de Bordeaux
2; ETS Franche Comté, Besançon; UMR 5533 CNRS, Pessac,
France; the Department of Medicine, the New York Hospital-Cornell
Medical Centre, New York, NY.
CD40 ligand (CD40L)/CD40 interactions play a central role in
T-cell-dependent B-cell activation as previously shown by in vitro
studies, the phenotype of CD40L knockout mice and the defective expression of CD40L in patients who have X-linked immunodeficiency with
hyper-IgM. The distribution of CD40 in cells other than of myeloid and
lymphoid lineages has suggested additional functions for this
receptor/ligand couple. Here we show that CD40L stimulates myelopoiesis
with a noticeable effect on megakaryocytopoiesis in cocultures of
hematopoietic progenitor cells and bone marrow stromal cells.
These results suggest a mechanism by which T-cell or
platelet-associated or soluble CD40L may regulate myelopoiesis.
(Blood. 2000;95:3758-3764)
The interaction of CD40 ligand (CD40L), a type II
transmembrane protein that is expressed on activated CD4+ T
lymphocytes, with its cognate receptor CD40, constitutively present on
B cells, is essential to the T-cell-dependent proliferation and
differentiation of B cells.1-3 This is strikingly
illustrated by the absence of germinal center, Ig isotype-switching,
and B-cell memory in patients who have hyper-IgM syndrome, resulting
from mutations in the CD40L gene and a subsequent lack of
expression of functional CD40L at the surface of activated T
cells.4-6 CD40 is also expressed on monocytes, macrophages,
dendritic cells, epithelial cells, fibroblasts, and endothelial cells
(ECs), suggesting that it has a broader function in vivo. For
example, CD40 triggering on these cells stimulates the production of
interleukin-6 (IL-6), IL-8, IL-1 As CD40L stimulates the release of cytokines such as GM-CSF, IL-6 or
LIF, we asked the question whether CD40L could be a regulator of
hematopoiesis through the regulation of hematopoietic growth factor
(HGF) biosynthesis by cells in the bone marrow and its environment. In this study, we present evidence that CD40L indirectly stimulates myelopoiesis with a noticeable effect on
megakaryocytopoiesis. The up-regulation of the production of
flt3-ligand (FL) and thrombopoietin (TPO) are instrumental and
essential to these actions.
Reagents
Stromal cells
Endothelial cells from the umbilical cord.
Primary cultures of human umbilical vein endothelial cells (HUVECs)
were obtained from freshly collected umbilical cords as originally
described.17 No exogenous growth factors were added.
Human bone marrow endothelial cell line.
The transformed bone marrow endothelial cell
(TrBMEC) line was derived from primary cultures of human
bone marrow endothelial cells (HBMECs) by intranuclear injection into
preconfluent cells of a DNA construct consisting of a portion of the
human vimentin promotor gene driving the SV 40 early genes (T and t
antigens).18 The cell line was maintained in IMDM
containing 5% fetal calf serum (FCS), glutathione, penicillin, and streptomycin.
Long-term bone marrow cultures.
Long-term bone marrow cultures (LTBMCs) were established in 25 cm2 tissue culture flasks from light-density bone marrow
cells. Low-density mononuclear cells were isolated by layering bone
marrow over Ficoll-Hypaque (density 1.077 g/cm,3 Seromed,
Biochrom KG, Berlin, Germany). Cells were grown in IMDM, supplemented
with 12.5% FCS, 12.5% horse serum, penicillin, streptomycin, and
10 Bone marrow-derived myofibroblastic cells.
Bone marrow-derived myofibroblasts were obtained as
described.19
CD34+ cell isolation and cocultures with endothelial
cells
Cytokine neutralization experiments Neutralizing polyclonal antibodies directed against IL-1 ,
IL-1 , IL-6, IL-11, G-CSF, GM-CSF, and M-CSF were purchased from R&D
systems (cat nos. AB-200-NA, AB-201-NA, AB-206-NA, AB-218-NA, AB-214-NA, AB-215-NA, and AB-216-NA, respectively). Neutralizing polyclonal anti-LIF antibody was a kind gift from V. Praloran, CHU
Dupuytren, Limoges, France. In preliminary experiments, 5 µg/mL final
concentration of each antibody were found to give an efficient
neutralization of a combination of recombinant human IL-1, IL-1,
IL-6, IL-11, G-CSF, GM-CSF, M-CSF, and LIF at concentrations of 50 ng/mL each.
Immunofluorescence Immunofluorescence for FL. Stromal cells were left to adhere to FCS-coated coverslips. They were then fixed with 4% paraformaldehyde for 10 minutes, washed 3 times with phosphate-buffered saline (PBS), and blocked for 45 minutes with 2.5% FCS in PBS. Then, cells were incubated with the monoclonal anti-FL antibody for 30 minutes at room temperature, washed, and incubated with secondary FITC-labeled antimouse antibody (Sigma) for 30 minutes at room temperature. Control coverslips were incubated with combinations of control isotypic antibodies at the same protein concentrations. Coverslips were mounted with antifade medium (Vectashield, Biosys, Compiègne, France), sealed, and examined under an Olympus AX 70 microscope (Scop SA, Rungis, France). Immunofluorescence for GPIIb/IIIa. Immunofluorescence was carried out on cytospins after liquid cultures. Cells were fixed and processed as above. Staining was performed with FITC-labeled anti-CD41 (Coulter-Immunotech, Marseille, France). Flow cytometry analysis Cells were labeled with the indicated FITC- or phycoerythrin (PE)-labeled monoclonal antibodies or with the corresponding isotypic controls for 30 minutes at 4°C in phosphate-buffered saline-bovine serum albumin (PBS-BSA) 1% and analyzed on an EPICS XL flow cytometer (Coultronics, Paris, France). Cells were phenotyped with the following mAb: SJ1D1 (anti-CD13, Coulter/Immunotech, Marseille, France), Leu-M9 (anti-CD33, Becton/Dickinson); Leu-M3 (anti-CD14, Becton/Dickinson); Leu-12 (anti-CD19, Becton/Dickinson); 69(Plt-1) (anti-CD41, Coulter/Immunotech); SZ21 (anti-CD61, Coulter); and Bear1 (anti-CD11b, Coulter/Immunotech). Ten thousand events were stored in list mode and analyzed using System II software (Coultronics).Western blotting HUVECs or LTBMCs were cultured 48 hours with 10% supernatant of nontransfected COS cells or with 10% supernatant of CD40L-CD8-transfected COS cells. The medium was then removed and
replaced by RPMI with or without CD40L and the incubation continued for
an additional 8 hours (to eliminate FCS that gives nonspecific signals
on the blots). The conditioned medium was concentrated 30-fold by
freeze-drying and analyzed by Western blotting according to standard
procedures. Briefly, samples were subjected to 7.5% SDS-PAGE and
electrotransferred to nylon membranes. Blots were developed using
anti-FL or anti-TPO antibodies (R&D systems, cat no. AF-308-NA and cat
no. AF-288-NA, respectively) and peroxydase-conjugated second antibody,
followed by chemiluminescence detection (Amersham, Little Chalfont,
UK). Recombinant human FL was a gift from Dr S. D. Lyman, Immunex Corp, Seattle, WA. Recombinant human TPO (carrier-free [cat no. 288-TP] [CF], as albumin gives nonspecific signal) was from R&D.
Cytokine measurements in culture medium Cells were cultured for 48 hours with 10% supernatant of nontransfected COS cells or with 10% supernatant of CD40L-CD8-transfected COS cells. The measurements of FL and TPO
levels in culture supernatants were performed using ELISA kits
purchased from R&D systems according to the manufacturer's
instructions. According to the manufacturer, the minimum detectable
dose of TPO is less than 15 pg/mL, the lowest TPO standard being 31.2 pg/mL.
Hematopoietic colony assay Colony assays were performed using either the Methocult GF+ H4435 (StemCell Technologies Inc, Meylan, France [this assay detects granulocytic-monocytic, erythroid, and multilineage colonies]), following the manufacturer's recommendations, or as previously described.20 Colony assays for megakaryocyte progenitors were performed using MegaCult-C (StemCell Technologies), following the manufacturer's recommendations. Staining of megakaryocyte progenitors was performed using a monoclonal antibody to GP IIb (anti-CD41 from Coulter-Immunotech or EDU-3, a monoclonal antibody recognizing a complex-dependent epitope on GP IIb-IIIa21). Bound primary antibody was detected using a biotin-conjugated secondary antibody and avidin alkaline-phosphatase, following standard procedures. Cell nuclei were counterstained with Evans blue.Statistics Results were expressed as the mean ± SD. Significant differences between values obtained in each assay were determined when applicable using the Wilcoxon signed rank test. Differences were considered as significant when P < .05.
CD40L enhances the proliferation and differentiation of
CD34+ progenitor cells toward the myeloid
lineage.
As illustrated in Figure 1, in cocultures
of CD34+ progenitor cells with ECs, the addition of CD40L
to the culture medium enhances the expansion of nucleated cells (Figure
1A) and the expansion of clonogenic cells (Figure 1B).
Stimulation of megakaryocytopoiesis.
The expanded cell population in the presence of CD40L essentially
belonged to the myeloid lineage (CD13, CD14, CD11b, CD33) and
surprisingly, a significant number of cells expressing megakaryocytic markers CD41 and CD61 (Figure 2A) were also
detected.
Enhancement of clonogenic cell generation by CD40L is dependent on the augmentation of FL biosynthesis. CD40L effects were indirectly mediated. First, we did not observe any significant direct effect of CD40L on the proliferation of CD34+ progenitors (not shown). Second, prestimulation of the EC monolayer for 48 hours with CD40L, followed by washing to remove CD40L before starting the coculture showed essentially the same results as those depicted in Figure 1. We therefore examined whether CD40L could modulate the expression of FL, a cytokine that has been shown to be of paramount importance in the proliferation of primitive hematopoietic cells.
CD40L stimulates megakaryocytopoiesis by way of the induced
production of TPO by stromal cells.
A finding of this study was that CD40L stimulated megakaryocytopoiesis.
In an effort to understand the molecular basis for this
megakaryocytopoiesis-promoting effect of CD40L, we measured the
production of TPO by stromal cells. Under basal conditions, the
concentrations of TPO were barely detectable, at the limit of ELISA
detection and accuracy (15-30 pg/mL) in all cell types tested. However,
CD40L induced production of TPO in all stromal cell types tested
(Figure 5A), results confirmed by Western
blotting that showed a moderate but consistent increase of TPO protein after stimulation (Figure 5B Western blot analysis of HUVEC- and LTBMC-conditioned medium). Neutralization of TPO in the CD40L coculture
system resulted in the inhibition of the capacity of stromal cells,
either ECs or LTBMCs to support the expansion of the
megakaryocyte progenitors, as demonstrated by flow cytometry experiments (illustrated in Figure 6: in
the presence of the anti-TPO antibody, there is a shift of the CD41
fluorescence to the level of the isotypic control), and colony assays
that showed a complete absence of megakaryocytic colonies after
neutralization of TPO (not shown). Neutralization of TPO did not affect
cell expansion, the colony number was reduced by an average of 18% (3 experiments). Neutralization of FL did not affect the number of
megakaryocytic colonies. This suggested that the increased production
of TPO by stromal cells in the presence of CD40L was the main cause for the increased generation of megakaryocyte progenitors.
In the CD40 coculture system, the proliferation
and differentiation of the hematopoietic progenitor cells are dependent
on the induction of cytokine biosynthesis by the stromal cells.
Activation of ECs, fibroblasts, or epithelial cells through their CD40
antigen has been shown to result in the increased production of
cytokines such as IL-6, IL-8, GM-CSF, G-CSF, or LIF.7-14 We
extend those conclusions by demonstrating the role of CD40 signaling in
the induction of FL and TPO biosynthesis.
J. Banchereau and Dr C. Van Kooten are gratefully acknowledged for
the gift of the CD40L cDNA.
Submitted March 23, 1999; accepted February 14, 2000.
Supported by the Ligue Nationale contre le Cancer.
Reprints: Jean Ripoche, UMR 5540 CNRS, Université de
Bordeaux 2, 146 rue Léo Saignat, 33076 Bordeaux, France; e-mail: jean.ripoche{at}umr5540.u-bordeaux2.fr.
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.
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Top
Abstract
Introduction
7 mol/L hydrocortisone (Sigma). Semiconfluent
stromal cell layers were trypsinized, replated in 6-well plates, and
grown until confluency. Cells were then washed to remove hydrocortisone
and incubated in IMDM with penicillin and streptomycin.
of all types tested
