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HEMATOPOIESIS
From the MGH Cancer Center and AIDS Research Center,
Massachusetts General Hospital, Harvard Medical School, Boston, MA, and
Radiation Oncology, University of Pittsburgh Cancer Institute,
Pittsburgh, PA.
The regulation of stem cell proliferation is a poorly understood
process balancing rapid, massive blood cell production in times of
stress with maintenance of a multipotent stem cell pool over decades of
life. Transforming growth factor Modulation between brisk expansion and
differentiation or quiescence and self-renewal defines essential
processes of stem cells. Understanding the mechanisms of stem cell
cycle regulation may guide methods for altering their cell-cycle
kinetics for purposes of stem cell expansion and genetic manipulation.
A subset of low-molecular-weight molecules that interact with
cyclin-dependent kinases (CDKs) to impair progression through G1 phase
of the cell cycle has been defined. These cyclin-dependent kinase
inhibitors (CDKIs) can be divided into 2 families: the Cip/Kip family
including p21Cip1/Waf1 (p21), p27Kip1 (p27),
and p57Kip2 (p57), which may interact with many CDKs, and
the INK4 family, p16INK4A (p16), p15INK4B
(p15), p18INK4C (p18), and p19INK4D (p19),
which specifically inhibit Cdk4 and Cdk6.1 Both have been
shown to have essential roles in arresting cell-cycle progression in a
number of model systems.2,3
A component of the quaternary complex, p21 is composed of cyclin D,
CDK4, and proliferating cell nuclear antigen.4 It is an
effector for p53-mediated cell-cycle arrest5 and is
transcriptionally regulated. We have demonstrated that restriction into
entry of the cell cycle in stem cells is governed by p21 in whose
absence the stem cell pool is larger, more actively cycling, and more sensitive to exhaustion. Dominant inhibitory control over stem cell
cycling exerted by p21 dictates the size and kinetics of the stem cell
compartment, and preserving the stem cell population is dependent on
restricting access to the cell cycle.6
P27 is molecularly distinct from p21 in its carboxyl terminus; it
interacts with similar, though not identical, cyclin-CDK and lacks p53
regulated expression.1,2,7 In addition, unlike p21, p27 is
controlled by translational and posttranslational mechanisms.8,9 A role for p27 in hematopoiesis is
supported by direct flow cytometric evidence for expression in
primitive cells10 and expression in more mature
progenitors,11,12 and indirectly it is supported by
improved retroviral transduction in the context of antisense
p27.13 We used mice engineered to be deficient in p27 to
define that p27 does not affect stem cell number, cell cycling, or
self-renewal but that it markedly alters progenitor proliferation and
pool size.14 Therefore, distinct CDKIs govern the highly
divergent stem and progenitor cell populations.
Transforming growth factor- Human bone marrow sampling and cell sorting
Murine bone marrow sampling and colony assay
32D cell line culture and synchronization The 32D cell line28 was maintained in 10% fetal calf serum supplemented with 10% WEHI-conditioned medium (used as the source for m-IL-3), and the medium was replaced twice weekly. WEHI-conditioned medium was withdrawn from the culture for 12 to 16 hours, and 70% to 80% cells were synchronized at G0/G1 phase as documented by propidium iodide analysis.293H-thymidine incorporation and cell-cycle analysis One microcurie 3H-thymidine (DuPont-New England Nuclear, Boston, MA) was added to 20 000 cells (200 µL) in 96-well plates, and cell mixture was incubated for 8 hours at 37°C. Thymidine-incorporated cells were harvested, filtered onto 96-well microfilter plates (Packard, Meriden, CT), and evaluated by liquid scintillation beta counter (Packard). Cell-cycle analysis was performed by standard propidium iodide staining and flow cytometry (Becton Dickinson) assessment of DNA content.Single-cell reverse transcription-polymerase chain reaction Single-cell reverse transcription-polymerase chain reaction (RT-PCR) was performed according to a minor modification of the method of Brady et al.30,31 Briefly, cells were lysed in 5.0 µL buffer (100 mM Tris HCl, pH 8.3, 150 mM KCl, 6 mM MgCl2, 4 µM each dNTP [Pharmacia], 100 ng/mL oligo (dT)24, 3360 U/mL RNA guard [Pharmacia], 100 U/mL Prime inhibitor [5 Prime-3 Prime, Boulder, CO], 20 mM dithiothreitol [DTT], and 0.5% NP-40). Samples were heated to 65°C for 1 minute, cooled to 22°C for 3 minutes, and put on ice. One hundred units of murine Moloney reverse transcriptase (Gibco-BRL) and 2 U Avian reverse transcriptase (Boehringer Mannheim) were added, and volume was made up to 10 µL with diethyl pyrocarbonate-treated H2O. Samples were incubated at 37°C for 20 minutes before heat inactivation at 65°C for 10 minutes. Resultant cDNA was then subjected to polyadenylate tailing in 20 µL total volume (50 mM Tris HCl, pH 8.3, 0.2 M potassium cacodylate, 5 mM CoCl2, 5 mM DTT, 250 µ/mL BSA, 0.2 mM dATP, and 10 U terminal transferase [Boehringer Mannheim]) at 37°C for 15 minutes, then heated at 65°C for 10 minutes and placed on ice. PCR was performed in a final volume of 50 µL (30 mM Tris HCl, pH 8.3, 65 mM KCl, 3.1 mM MgCl2, 1 mM each dNTP, 100 µ/mL BSA, 0.05% Triton X-100, 10 µM (dT) 24-primer, and 5 U AmpliTaq polymerase [Perkin-Elmer]). Cell-free and reverse transcriptase-free samples were used as negative controls. Samples were initially amplified for 25 cycles of 30 seconds at 94°C, 1 minute at 42°C, and 3 minutes (plus 5-second extension cycle) at 72°C in a thermal cycler (9600 model; Perkin-Elmer Cetus). An additional 5 U Taq polymerase was then added, and another 25 cycles were performed.Southern blotting The PCR product was electrophoresed through 1.2% agarose, stained with ethidium bromide, photographed, transferred to a nylon membrane (Micron Separations) with vacuum blotter (Pharmacia), immobilized by UV (Stratagene), and hybridized to the indicated 32P-radiolabeled probes (1 × 107 cpm/mL) with the use of 40 bp 3'-oligodeoxyribonucleotides derived from the following human cDNA sequences: p21Cip1/Waf1, p27Kip1, TGF- 1, and TGF-1 receptor (type II)
(hereafter referred to TR II) in the ExpressHybridization Solution
(Clontech). The hybridization temperature for the oligo probes was
37°C, and final wash conditions were 0.1 × SSC and 0.1% sodium
dodecyl sulfate (SDS) at 37°C. Hybridized blots were analyzed by
PhosphorImager (Molecular Dynamics) quantitation and autoradiography.
RNA isolation and Northern blotting Total RNA was isolated from the cells using the guanidine isothiocyanate procedure coupled with ultra-centrifugation through the CsCl2 cushion. Equal amounts (10 µg) total RNA were analyzed on formaldehyde gels and blotted onto nylon membrane (Micron Separations) using a commercial UV cross-linker (Invitrogen). The cDNA probes were labeled by 32P using the random primer extension system (DuPont-New England Nuclear) with 68°C hybridization temperature for the cDNA probes in the Express Hybridization Solution (Clontech). Final wash conditions were 0.1 × SSC and 0.1% SDS at 55°C. Hybridized blots were analyzed by PhosphorImager (Molecular Dynamics) quantitation and autoradiography. Mouse p21 and p27 cDNA plasmids were kindly provided by Dr David Beach (Cold Spring Harbor Laboratory).Western blotting 32D cells were lysed in lysis buffer (250 mM NaCl, 50 mM HEPES, pH 7.0, 0.1% NP-40, 50 mM NaF, 5 mM EDTA, pH 8.0, 100 mM sodium orthovanadate, 1 mg/mL leupeptin, 1 mg/mL aprotinin, 1 M DTT, and 50 mM phenylmethylsulfonyl fluoride), and equal amounts (30 µg) protein lysates were fractionated on a 12% SDS-polyacrylamide gel. Fractionated proteins were electrotransferred onto the nitrocellulose membrane (Millipore). The blocked protein blot was incubated with the rabbit anti-mouse p21 or p27 (Pharmingen) at the 1 µg/mL final concentration in Tris-buffered saline (TBS/T) (1 M Tris, pH 8.0, 5 M NaCl, 0.05% Tween 20) with 0.5% milk for more than 1 hour, rinsed with TBS/T buffer, and incubated with goat anti-rabbit IgG conjugated with horseradish peroxidase in the TBS/T. After washing, enhanced chemiluminescence (DuPont-New England Nuclear) was performed according to instructions from the manufacturer.
The hypothesis that TGF- P21 up-regulation during the terminal differentiation of primary hematopoietic cells P21 is primarily regulated at the transcription level,3,32-35 in contrast to other CDKIs, which are largely controlled by translational and posttranslational mechanisms.2,8,9 We evaluated the temporal expression pattern of p21 in the terminal differentiation of human primary hematopoiesis using RT-PCR analysis during the differentiation of the myeloid progenitor cell, macrophage-monocyte colony-forming unit (CFU-M). CD34+CD38 cells were plated at
limiting dilution in the medium for CFU-M development, and single
daughter cells from the same original progenitor were removed by
micromanipulation for subsequent analysis. During CFU-M development,
p21was almost undetectable at day 3 and was up-regulated after day 7. When normalized for glyceraldehyde-3-phosphate dehydrogenase
(GAPDH) expression, the up-regulation of p21 mRNA level was
highly time dependent (Figure 1). P21
expression achieved maximal levels by day 10, when the cells achieved
fully mature morphologic features and the characteristic gene
expression of a terminally differentiated monocyte previously
defined.30
Distinct expression profiles of p21 and p27 in hematopoietic cells Noting the up-regulation of p21 in terminally differentiated cells, we next evaluated stem cells at the opposite end of the differentiation schema that were also quiescent. We stimulated CD34+ cells with SCF-IL-3 while maintaining high concentrations of the S-phase-specific toxin 5-flurouracil and collected the remaining viable cells at day 7 by flow cytometry.27 Cells isolated using this technique have low staining for the mitochondrial staining dye pyronin Y and the DNA staining dye Hoechst 33342, consistent with the G0 phase of the cell cycle. We and others have shown that these cells have stem cell-like characteristics, as indicated by LTC-IC assays and hu-SCID repopulating experiments.27,36,37 Individual G0 cells were sorted as were other hematopoietic cells at different stages of development, characterized by immunophenotypic profiles including CD34+CD33 and
CD34+CD33+ from bone marrow and
CD11b+ and CD19+ from peripheral blood. Using
semiquantitative single-cell RT-PCR, we found that G0 cells
expressed high levels of p21 (Figure 2). In contrast, p27 was expressed relatively evenly in all the populations tested without a pattern of altered transcript levels (Figure 2). The
expression patterns of the genes tested in G0 were more uniform than others, perhaps reflecting the relative homogeneity of
G0 cells. In the CD34+CD33 subset
that represents early myeloid progenitors with high proliferative status, there was a very low or undetectable level of p21. In other
subsets of maturing (CD34+CD33+) and fully
matured (CD11b+) cells of myeloid lineage, there were
elevated levels of p21 (more than 2-fold by densitometry quantitation)
compared to CD34+CD33. Heterogeneity in
expression patterns within the CD34+ CD33+ and
CD11b+ populations likely reflects intrinsic variability in
those populations. Data in these 3 subsets were consistent with the
result of CFU-M as shown above (Figure 1) and support the association
of p21 transcription levels, with the state of differentiation
up-regulated in quiescent primitive cells or fully mature cells.
Because p27 is mainly regulated at the posttranscriptional level, data
on p27 mRNA level are less informative than for p21.
Expression of TGF- 1 participates in
the quiescence of primitive hematopoietic
cells.17,20,38,39 We evaluated the mRNA levels of TGF-1
and its receptor in G0 stem cells and the subsets of
differentiation stage-specific cells described above. TR II was
expressed throughout the cell types tested with a relatively stable
expression pattern (Figure 3). In
contrast, TGF-1 was expressed at high levels at the stage of
G0 stem cells and in fully mature cells. Therefore,
TGF-1 had an expression pattern similar to p21, consistent with
coordinate regulation (Figure 3). This supported the possibility that
p21 may be a downstream mediator of TGF-1's effects on cell
cycling, as has been documented in nonhematopoietic and transformed
cell systems.23-25,40
The induction of cell-cycle arrest by TGF-
The inhibitory effect of TGF- 1 on hematopoietic cells may not be mediated through p21 or p27. To further confirm this conclusion in
primary cells, mononuclear bone marrow cells were harvested from either
wild-type mice (+/+) or mice engineered to be deficient in p21
(p21 /) or p27 (p27/). The 8- to 10-week-old animals were
derived from the same heterozygous parents and analyzed for p21 or p27
genotype by tail clip DNA PCR. Animals from the same parent pairs were
used to avoid breeding-induced artifacts. CFC assays were performed in
standard methylcellulose cultures. Total CFCs were scored at day 10 to
assess progenitor pool activity and long-term culture with limiting
dilution (CAFC) to assess primitive cell activity. Although TGF-1
had a dose-dependent inhibitory effect on CFCs, the effect was not
different for either / cells or +/+ cells (Figure
8). In addition, 10 ng/mL TGF-1 was
able to completely inhibit the proliferation of stem cells (CAFCs) of
both genotypes (data not shown). These data demonstrate that TGF-1
mediates antiproliferative effects independent of p21 or p27 in
primitive hematopoietic cells.
TGF- We found that quiescent primary human stem cells express high levels of
p21, consistent with the functional data generated from
p21 The inhibitory role for p21 is more clearly defined and has been shown in numerous settings.49,50 When we evaluated quiescent primitive cells or terminally differentiated monocytic cells in the experiments reported here, we noted markedly elevated levels of p21 message. However, it should be noted that the association of increased p21 and terminal differentiation was cell type specific; we did not note a similar pattern in differentiating granulocytic cells (data not shown). This may also explain the insignificant change in the p21:GAPDH ratio we observed when examining CD34+ CD33+ versus CD11b+ cells because the latter includes a mixture of monocytic and granulocytic cells predominated by granulocytes (Figure 2). Taken together, p21 appears to have a dual function in the hematopoietic system depending on the differentiation stage and cyclin-CDK complex status. The coordinate expression of TGF- These data demonstrate that though TGF- Taken together, our data and the studies noted above support the
independence of the TGF- Our data leave unresolved what extracellular signals may modulate p21
and p27, known to be critical for controlling hematopoietic populations. Examples of possible other signals include interferon-
We thank Dr Tyler Jacks for providing p21+/
Submitted May 30, 2001; accepted August 9, 2001.
Supported by National Institutes of Health grants HL44851, DK50234, HL55718 (D.T.S.), and KO8 DK02761 (T.C.); the Richard Saltonstall Charitable Foundation (D.T.S.); and the Deutsche Akademischer Austauschdienst (S.S.).
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: David T. Scadden, Massachusetts General Hospital, Bldg 149, Rm 5212, 13th St, Charlestown, MA 02129; e-mail: scadden.david{at}mgh.harvard.edu.
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| Copyright © 2001 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
1 mediates cell-cycle arrest of
primitive hematopoietic cells independent of p21Cip1/Waf1
or p27Kip1
Top
Abstract
Introduction
-MEM semisolid matrix
culture medium (Stem Cell Technologies, Vancouver, BC, Canada) with
cytokine combinations of 50 ng/mL mu-SCF (R&D System), 20 ng/mL
m-IL-3 (R&D Systems), 20 ng/mL hu-IL-6 (R&D Systems), and 2 U/mL hu-erythropoietin (Amgen, Thousand Oaks, CA). Cells were plated at
20 000/200 µL/well into 48-well plates and were placed at 37°C,
5% CO2. At day 10, myeloid and erythroid colonies were
scored, totaled, and reported as colony-forming cells (CFCs)
representing committed progenitor cells.
, noted to induce p21 through STAT1 signaling in A431 epidermoid carcinoma cells,