Previous Article | Next Article 
Mol Cell Biol, May 1998, p. 2462-2473, Vol. 18, No. 5
Fox Chase Cancer Center, Philadelphia,
Pennsylvania 19111,1 and
University of
Pennsylvania School of Medicine, Philadelphia, Pennsylvania
191042
Received 23 September 1997/Returned for modification 30 October
1997/Accepted 1 February 1998
Gfi-1 is a cellular proto-oncogene that was identified
as a target of provirus integration in T-cell lymphoma lines selected for interleukin-2 (IL-2) independence in culture and in primary retrovirus-induced lymphomas. Gfi-1 encodes a zinc finger
protein that functions as a transcriptional repressor. Here we show
that Gfi-1B, a Gfi-1 related gene expressed in
bone marrow and spleen, also encodes a transcriptional repressor.
IL-6-induced G1 arrest and differentiation of the
myelomonocytic cell line M1 were linked to the downregulation of Gfi-1B
and the parallel induction of the cyclin-dependent kinase inhibitor
p21WAF1. Experiments addressing the potential
mechanism of the apparent coordinate regulation of these genes revealed
that Gfi-1B represses p21WAF1 directly by
binding to a high-affinity site at Hematopoiesis is a process that
takes place in the bone marrow throughout the life of an individual.
During this process a small number of hematopoietic stem cells respond
to microenvironmental cues to either divide and self-renew or
differentiate into hematopoietic progenitors committed to specic
hematopoietic lineages. The committed hematopoietic progenitors,
in turn, also undergo self-renewal or terminal differentiation. The
maintenance of the hematopoietic stem cells and their selection,
commitment, and maturation along different hematopoietic lineages
depend on cell-to-cell and cell-to-stroma interactions, secreted
cytokines, and intracellular signaling molecules (45, 46).
The molecular mechanisms involved in regulating hematopoietic cell
commitment and differentiation can be addressed in differentiating
hematopoietic tissues in intact animals (64) and in cell
lines that can be induced to differentiate (35, 38). With
both systems, a number of molecules, including growth factors,
receptors, and transcription factors, have been identified and shown to
contribute to hematopoiesis in a hierarchical order (10, 29, 42,
65).
The myelomonocytic cell line M1 undergoes G1 arrest and
differentiation following exposure to interleukin-6 (IL-6) or leukemia inhibitory factor (15, 50). During this process the
expression of several signaling molecules is altered. c-myb
is downregulated within 3 h from the start of the exposure to IL-6
or leukemia inhibitory factor (26). This is followed by the
downregulation of c-myc (25). Overexpression
of either c-myb or c-myc inhibits IL-6-induced
differentiation of M1 cells (25, 26, 49), suggesting that
the downregulation of these molecules is required for differentiation. Another molecule whose expression changes during differentiation of the
M1 cells is the cyclin-dependent kinase inhibitor
p21WAF1, which is induced following exposure to
IL-6 (57). One factor known to induce
p21WAF1 is p53 (12). Since M1 cells,
however, do not express p53 (62), the induction of
p21WAF1 in these cells is p53 independent.
Evidence presented in this report indicates that the p53-independent
induction of p21WAF1 in differentiating M1 cells
depends on the downregulation of the Gfi-1 homolog Gfi-1B, which
functions as a direct repressor of p21WAF1.
Gfi-1 is a cellular proto-oncogene that was identified as a
target of provirus integration in retrovirus-induced T-cell-lymphoma lines selected for IL-2 independence in culture and in primary retrovirus-induced lymphomas (16, 47, 48). Our early studies have shown that Gfi-1 encodes a transcriptional repressor
(66) whose repressor function depends on a novel repressor
domain SNAG (19). Forced expression of Gfi-1
inhibits apoptosis of primary thymocytes and immortalized T cells
(20) and abrogates G1 arrest induced by IL-2
withdrawal from IL-2-dependent T-cell lines (16, 20).
Gfi-1B was cloned by low-stringency hybridization to a probe
derived from the Gfi-1 zinc finger region. Interestingly, Gfi-1B was also found to be a target of provirus integration
in a subset of B-cell lymphomas induced by Moloney murine leukemia virus (Mo-MuLV) in Eµ-myc transgenic,
pim-1/pim-2 knockout mice (39a).
Here we show that Gfi-1B also encodes a SNAG domain
containing a transcriptional repressor and that the
p21WAF1 promoter is one of its direct targets.
IL-6 treatment of M1 cells results in the downregulation of
Gfi-1B and the parallel induction of
p21WAF1. The induction of
p21WAF1 is a direct consequence of the
downregulation of Gfi-1B. Inhibition of the induction of
p21WAF1 by the forced expression of
Gfi-1B inhibits cell cycle arrest and differentiation
of the M1 cells, suggesting that these processes depend on
p21WAF1 expression. Although
p21WAF1 expression can be induced by a multitude
of transcriptional activators (5, 8, 21, 36, 37, 43, 44, 54-56,
58, 64), Gfi-1B appears to be its only repressor known to date.
(This work was carried out to partially fulfill the Ph.D. thesis
requirements of B.T. at the University of Pennsylvania School of
Medicine.)
Isolation and sequencing of Gfi-1B cDNA.
A 2.9-kb
EcoRI fragment from rat genomic DNA hybridizing to a DNA
probe from the zinc finger region of the rat Gfi-1 gene (40% formamide, 6× SSC [1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate] at 37°C) was cloned into the lambda phage vector lambda ZapII (Stratagene). A 400-bp, repeat-free PstI fragment
isolated from this clone was hybridized to RNA from different mouse
tissues and was shown to be expressed primarily in spleen and bone
marrow. Screening a murine spleen cDNA library (Stratagene) with the
same probe identified seven cDNA clones representing a novel
Gfi-1-related gene which was named Gfi-1B. The
pBluescript(SK Northern and Western blotting.
RNA was isolated from
different mouse tissues or cultured cells by the method of Chomczinski
and Sacchi (9). Total RNA (15 µg) was electrophoresed in
1% formaldehyde agarose gel. Following transfer to Hybond-N nylon
membranes (Amersham), the RNA was hybridized to DNA probes as described
in the Results section.
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
The Gfi-1B Proto-Oncoprotein Represses
p21WAF1 and Inhibits Myeloid Cell
Differentiation
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
1518 to 1530 in the
p21WAF1 promoter. Forced expression of
Gfi-1B, but not of Gfi-1B deletion mutants lacking the
repressor domain, blocked the IL-6-mediated induction of
p21WAF1 and inhibited G1 arrest and
differentiation. We conclude that Gfi-1B is a direct repressor of the
p21WAF1 promoter, the first such repressor
identified to date, and that sustained expression of Gfi-1B blocks
IL-6-induced G1 arrest and differentiation of M1 cells
perhaps because it prevents p21WAF1 induction
by IL-6.
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
)/Gfi-1B plasmids generated by in vivo excision
(according to the manufacturer's protocol) were subjected to sequence
analysis (Sequenase kit; U.S. Biochemical Corp.) with vector- and
Gfi-1B-specific oligonucleotide primers. The sequences
obtained were analyzed with the GCG sequence analysis software package
(Genetics Computer Group, Madison, Wis.).
Bacterial GST-Gfi-1B fusion protein and Gfi-1B DNA binding: random oligonucleotide selection. To express the Gfi-1B zinc finger domain in E. coli, we amplified the associated DNA sequence by PCR. BamHI and EcoRI restriction sites were introduced at the ends of the amplified DNA, which was then digested with BamHI and EcoRI and subcloned in frame with glutathione S-transferase (GST) in the pGEX vector (Pharmacia).
Bacterial cells transformed with the resulting expression construct pGEX-Gfi-1B were grown to log phase and induced with 1 mM isopropyl-
-D-thiogalactopyranoside (Sigma). At 2 h
following induction, the bacteria were pelleted and sonicated in
ice-cold phosphate-buffered saline (PBS) containing the protease
inhibitor phenylmethylsulfonyl fluoride (PMSF) (Sigma) (1 mM). The
lysates were then clarified by centrifugation at 15,000 × g and mixed with glutathione-linked agarose beads (Sigma).
To identify the DNA-binding consensus for Gfi-1B, a random
double-stranded oligonucleotide pool was generated as described previously (66). A 1-µg portion of the mixture of
double-stranded oligonucleotides containing an 18-bp random sequence at
the center was incubated with 5 µg of the GST-Gfi-1B fusion protein
attached to glutathione-linked agarose beads. Incubation was
carried out at 25°C in binding buffer (25 mM HEPES [pH
7.5], 100 mM KCl, 0.1 mM ZnSO4, 10 mM MgCl2, 0.1% Nonidet
P-40, 1 mM dithiothreitol [DTT], 5% glycerol, poly[dI-dC]
[0.2 mg/ml], bovine serum albumin [0.2 mg/ml]) for 30 min. The
beads were then centrifuged and washed three times with binding
buffer and then boiled for 5 min in water. The oligonucleotide mixture
eluted by boiling was used as a template for PCR amplification. After
four rounds of selection and amplification, the PCR products were
cloned into pBluescript. Plasmid DNA from 80 individual E. coli transformants was sequenced to determine the binding
consensus for Gfi-1B.
Cell lines and cultures. M1 cells (TIB 192) and NIH 3T3 cells (TIB 163) were obtained from the American Type Culture Collection (Rockville, Md.), while the 10-1 cells (23) were provided by J. Sherley (Fox Chase Cancer Center). 10-1 cells and NIH 3T3 cells were grown in Dulbecco modified Eagle medium supplemented with 10% fetal bovine serum and 1% penicillin, 1% streptomycin, and 1% kanamycin, while M1 cells were grown in RPMI supplemented with 10% endotoxin-free fetal bovine serum (Gibco BRL) and 1% penicillin, 1% streptomycin, and 1% kanamycin. M1 cells were seeded at 2 × 105 cells per ml prior to exposure to murine recombinant IL-6 (50 ng/ml) (R&D Systems).
Expression and reporter constructs.
To generate
pCMV5/Gfi-1B, the 1.7-kb full-length Gfi-1B cDNA was
released from pBluescript(SK) by double digestion with
EcoRI and SalI and then subcloned between
EcoRI and SalI in the CMV5 expression vector
(1) or between EcoRI and XhoI in the
expression vector pcDNA3 (Invitrogen).
SNAG mutant (which lacks the first 20 amino acids of
Gfi-1B), an oligonucleotide homologous to the zinc finger region 3'
of the HindIII site at nucleotide 765 and another
oligonucleotide containing an EcoRI restriction site, the
Gfi-1B ATG, and 15 nucleotides encoding amino acids 21 to 25 of
Gfi-1B were used in an amplification reaction with the Gfi-1B cDNA
as template. The product of the reaction was digested with
EcoRI and HindIII and ligated into a
pDNA3-based construct containing the zinc finger region of the Gfi-1B
cDNA from the HindIII site to the unique
BamHI site at nucleotide 1390 in the 3'-untranslated region
of the gene. The delta amino terminus (Nter) construct was made in a
similar manner with the same first oligonucleotide (in the zinc finger
region) and another oligonucleotide containing an EcoRI
restriction site, the Gfi-1B ATG, and 15 nucleotides encoding amino
acids 164 to 168. The product of the amplification reaction was
digested with EcoRI and HindIII and ligated
into a pDNA3-based construct containing the
HindIII-to-BamHI fragment of
Gfi-1B. All clones were sequenced to ensure that the final product
contained no additional mutations.
Transfections. NIH 3T3 cells were transiently transfected using Lipofectamine reagent (Gibco BRL) as suggested by the manufacturer. About 1.8 × 105 cells were seeded in 35-mm-diameter petri dishes 16 h prior to transfection. Reporter plasmids (1.8 µg) and 100 ng of pCMV5 empty vector, pCMV5/Gfi-1B, or pCMV5/VP16/Gfi-1B were cotransfected.
10-1 cells were transfected by the calcium phosphate precipitation method (17). About 3.5 × 105 cells were seeded in 60-mm-diameter petri dishes prior to transfection. Portions (1.5 µg) of different p21WAF1 promoter constructs and 3 µg of pCMV5/Gfi-1B or 0.25 µg of p21WAF1 promoter constructs and 4.25 µg of pCMV5/VP16/Gfi-1B were cotransfected. Stable transfections were performed by electroporation (19). pcDNA3 empty vector and pcDNA3/Gfi-1B were prepared with Qiagen columns (QIAGEN, Inc.). The plasmid DNAs were gel purified following linearization by EcoRI digestion. M1 cells were seeded 16 h prior to transfection. Electroporation of 107 M1 cells, suspended in 250 µl of medium (without antibiotics), was carried out in 0.45-µm cuvettes (Bio-Rad) with 20 µg of DNA. Samples were pulsed at 960 µF and 260 mV and placed in culture for 48 h before selection. The cells were then diluted and seeded at 5 × 104 cells per ml in growth medium containing 400 µg of geneticin per ml (G418 sulfate; Gibco BRL) and divided into aliquots in 24-well plates (5 × 104 cells/well). After 3 to 4 weeks, cultures from wells containing surviving cells were expanded and subcloned in agar in the presence of G418. The Gfi-1B/SNAG and Gfi-1B/Nter transfectants
were maintained as mass cultures. Fully selected transfectants were maintained in G418 at 200 µg/ml.
Chloramphenicol acetyltransferase (CAT) assays.
NIH 3T3 or
10-1 cells were cotransfected with Gfi-1B, VP16/Gfi-1B, and CAT
reporter constructs as described above. Cell lysates were collected
40 h later by four consecutive freeze-thaw cycles and were
normalized for transfection efficiency by a -galactosidase assay
(6). Lysates were analyzed for CAT activity by thin-layer chromatography (61).
In vitro translation, preparation of M1 nuclear extracts, and electrophoretic mobility shift assays (EMSAs). Gfi-1B was in vitro transcribed and translated by the TNT T7-coupled reticulocyte lysate system (Promega). Nuclear extracts were prepared from untreated and IL-6-treated M1 cells collected at 36 h after the start of the IL-6 treatment by the protocol of Kramer and Keller (30). Briefly, 1 × 108 to 2 × 108 cells were collected in 25 ml of cold PBS and pelleted. After being washed with 1 ml of buffer A [10 mM HEPES-KOH (pH 7.9), 1.5 mM MgCl2, 10 mM KCl, 0.5 mM DTT], the cells were resuspended in 0.5 ml of the same buffer and they were forced several times through a 25-gauge-by-0.625-inch hypodermic needle. Collected cell nuclei were resuspended in 0.2 ml of buffer C (20 mM HEPES-KOH [pH 7.9], 25% glycerol, 0.42 M NaCl, 1.5 mM MgCl2, 0.2 mM EDTA, 0.5 mM phenylmethylsulfonyl fluoride, pepsin [1 µg/ml]). The nuclear extracts were dialyzed against 400 ml of buffer D [20 mM HEPES-KOH (pH 7.9), 20% glycerol, 0.1 M NaCl, 0.2 mM EDTA, 0.5 mM DTT]. The protein concentration of the nuclear extracts was determined by the Bradford assay (Bio-Rad).
EMSAs were done with a double-stranded oligonucleotide probe containing the Gfi-1B binding site (5'-CCGAAGTACCGTGATTTCAGGCATGCAC-3', annealed to its complementary strand). A mutant oligonucleotide (AATC to GGTC) was also generated. The wild-type double-stranded oligonucleotides were end labeled with [
-32P]ATP and T4 polynucleotide kinase (New England
Biolabs). One-tenth of the Gfi-1B translated in vitro from RNA derived
from 1 µg of pcDNA3/Gfi-1B or 12 µg of M1 nuclear extracts was
incubated with 104 cpm of the end-labeled oligonucleotides
(20 min at room temperature) in a 20-µl final volume in binding
buffer [12 mM HEPES (pH 7.6), 12% glycerol, 4 mM Tris, 60 mM KCl, 1 mM EDTA, 1 mM DTT, poly(dI-dC) (2 µg)]. To compete the
protein binding, excess wild-type or mutant double-stranded
oligonucleotides were incubated with the in vitro-translated product
(100- to 200-fold) or the M1 nuclear extracts (100-fold) for
15 min prior to the addition of the labeled probe. Samples were then
electrophoresed at 25 mA in nondenaturing polyacrylamide gels at 4°C
for 3 h in 0.5× TBE buffer (45 mM Tris-borate-1 mM EDTA [pH
8.0]) (66).
Cell cycle analysis. Parental M1, M1/vector, and M1/Gfi-1B cells were seeded at 2 × 105 cells per ml. After IL-6 treatment (50 ng/ml), the cells were harvested at sequential time points as indicated below. Harvested cells were washed with PBS and resuspended in fluorescence-activated cell sorter buffer (3.4 mM sodium citrate, 10 mM NaCl, 0.1% Nonidet P-40, 75 µM ethidium bromide) (51). The DNA content of these cells was then determined by flow cytometry. The data were analyzed with the CellQuest package (Becton Dickinson).
M1 cell attachment to the surface of the petri dish. Parental M1, M1/vector, and M1/Gfi-1B cells were seeded at 2 × 105 cells per ml, and they were treated with IL-6 (50 ng/ml). After 48 h, the medium and the suspension cells were removed, the dishes were washed twice with PBS, and the cells were photographed with an inverted microscope (Nikon).
Mac-1 expression.
Parental M1, M1/vector, and M1/Gfi-1B
cells were collected at 96 h following IL-6 treatment. Expression
of Mac-1 was then determined by staining the cells with the anti-mouse
CD11b monoclonal antibody M1/70 (Pharmigen), which is directed against
the Mac-1 
m chain. This chain is known to be induced during
differentiation along the macrophage lineage (4). Stained
cells were analyzed by flow cytometry with a fluorescence-activated
cell sorter and the CellQuest software package (Becton Dickinson).
Nucleotide sequence accession number. The cDNA sequence for Gfi-1B has been submitted to GenBank under accession no. AF017275.
| |
RESULTS |
|---|
|
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
|
|---|
Gfi-1B encodes a Gfi-1-related zinc finger protein that is expressed in bone marrow and spleen. With a DNA probe derived from the zinc finger region of Gfi-1 (16) and low-stringency hybridization, we cloned three novel zinc finger protein-encoding genes from rat DNA. A full-length cDNA clone of one of these genes, Gfi-1B, isolated from a murine spleen cDNA library (Stratagene), encodes a 330-amino-acid zinc finger protein which is 97% identical to Gfi-1 in the zinc finger region. The homology between the two proteins, amino-terminal to their zinc finger domains, is restricted to a 20-amino-acid peptide which defines the Gfi-1 repressor domain SNAG (19) (Fig. 1A). SNAG is shared by Gfi-1 and Gfi-1B, the members of the Snail/Slug family of proteins found in vertebrates (19), the zinc finger protein IA-1, which is overexpressed in neuroendocrine neoplasms (32), and the homeobox protein Gsh-1, which is involved in pituitary development (34).
|
Gfi-1B is a sequence-specific DNA-binding protein that functions as a transcriptional repressor. The sequence homologies between Gfi-1B and Gfi-1 suggested that the latter may also be a sequence-specific DNA-binding protein and that it may also function as a transcriptional repressor. To address the first hypothesis, we used the random oligonucleotide binding and selection strategy (66). The oligonucleotide library selected after four rounds of Gfi-1B binding was cloned into pBluescript, and the isolated clones were sequenced. Of 80 sequenced clones, all contained at least one AATC motif. Aligning the sequences of 64 clones with one or two AATC motifs revealed that the Gfi-1B DNA-binding consensus sequence (Fig. 2 and Table 1) is virtually identical to the DNA-binding consensus sequence of Gfi-1 (66). To examine whether Gfi-1B also functions as a transcriptional repressor, NIH 3T3 cells, which express neither Gfi-1 nor Gfi-1B (data not shown), were cotransfected with a CMV5/Gfi-1B expression construct and a CAT reporter construct. The CAT gene in the latter construct was under the control of a minimal thymidine kinase promoter from herpes simplex virus with one to four concatamerized Gfi-1/Gfi-1B binding sites upstream or four sites downstream of the reporter (19). Alternatively, this construct contained a single mutant site (GATC as opposed to AATC) upstream of the reporter (Fig. 3A). The results (Fig. 3C, upper panel) showed that Gfi-1B represses all constructs containing wild-type Gfi-1B binding sites but has no effect on the construct containing the mutant site. The strength of the repression was proportional to the number of Gfi-1B binding sites in the reporter construct. Cotransfection of the same reporter constructs with an expression construct of a VP16/Gfi-1B chimera (Fig. 3B) revealed that the chimera activates the reporters that are repressed by wild-type Gfi-1B (Fig. 3C, middle panel). These results collectively indicate that Gfi-1B is an additive, distance-independent, active transcriptional repressor which functions by binding to the same DNA sequence as Gfi-1.
|
|
|
G1 arrest and differentiation induced by exposure of the myelomonocytic cell line M1 to IL-6 depend on the IL-6-induced downregulation of Gfi-1B. Both Gfi-1B and Gfi-1 are expressed in the bone marrow. However, the two genes are differentially expressed in the cells that leave the bone marrow to populate the thymus and the spleen. Thus, thymocytes express mainly Gfi-1, while splenocytes express almost exclusively Gfi-1B (Fig. 1B). Additional hematopoietic-lineage-specific expression studies showed that Gfi-1B is expressed in early hematopoietic cells and that its expression declines with differentiation (44a).
This pattern of expression suggested that Gfi-1B may be involved in the differentiation of hematopoietic cells. To test this hypothesis we first examined whether IL-6-induced differentiation of the myelomonocytic cell line M1 is associated with changes in Gfi-1B expression. The results showed that growing M1 cells express substantial levels of Gfi-1B and that Gfi-1B expression declines to undetectable levels within 24 h, following exposure to IL-6 (Fig. 4Aa, left panel). The downregulation of Gfi-1B could either be the cause or the result of differentiation. To distinguish between these possibilities, we examined whether forced expression of Gfi-1B inhibits IL-6-induced differentiation. Gfi-1B was stably transfected into M1 cells by using a pcDNA3 expression construct. Of 20 transfected M1 cell clones, 3 overexpress Gfi-1B as determined by the sustained expression of the gene following exposure of the clones to IL-6. Fig. 4Aa (right panel) shows the expression of Gfi-1B in one of these clones before and 24 h after the start of IL-6 treatment. Fig. 4Ba shows a dot blot analysis of RNA isolated from wild-type and vector-transfected M1 clones (blots 1 and 2, respectively) and four Gfi-1B-transfected clones at 24 h after exposure to IL-6. Of the latter clones, one (blot 3) does not express Gfi-1B constitutively, whereas the other three (blots 4, 5, and 6) do. The same cell clones were then scored for IL-6-induced differentiation, which was measured by their relative attachment to the surface of the petri dish at 48 h and by the relative expression of Mac-1, a marker of mature macrophages, granulocytes, and natural killer cells (2) at 96 h following exposure to IL-6. Mac-1 expression was determined by immunofluorescence staining and flow cytometry (4). The results revealed that forced expression of Gfi-1B prevented both cell attachment (Fig. 4Bb1) and Mac-1 induction (Fig. 4Bc1). Clone 3, however, which had been transfected with the Gfi-1B construct but did not overexpress Gfi-1B, underwent differentiation in a way similar to that of the parental and vector-transfected cells. Identical results were obtained with three mass cultures of M1 cells infected with the MSCV retrovirus vector (24) or MSCV-based Gfi-1B expression constructs (data not shown).
|
SNAG and Gfi-1BNter. These Gfi-1B mutants harbor deletions
of the SNAG domain (amino acids 2 to 20) or the entire amino-terminal region (amino acids 2 to 163), respectively, and lack transcriptional repression activity (59). The transfected cells were then
treated with IL-6, and they were examined at the indicated time points for Gfi-1B expression, differentiation, and cell cycle distribution. Expression of Gfi-1B was determined by Northern blotting,
differentiation was determined by cell attachment to plastic, and Mac-1
expression and cell cycle distribution were determined by flow
cytometry as described above. The results (Fig. 4) revealed that
Gfi-1BSNAG and Gfi-1BNter fail to inhibit the IL-6-induced
G1 arrest and differentiation of M1 cells. Therefore, the
effects of Gfi-1B on IL-6-induced cell cycle arrest and differentiation
of the M1 cells depend on its ability to repress transcription.
Epistatic relationship of the downregulation of Gfi-1B, c-myc, and c-myb during IL-6-induced differentiation of M1 cells. At least two other oncogenes, c-myb and c-myc, are known to be downregulated during IL-6-induced differentiation of the M1 cells and their downregulation is necessary for differentiation (25, 26). To map the action of Gfi-1B epistatically relative to c-myb and c-myc, parental as well as vector or Gfi-1B-transfected M1 cells were examined for c-myb or c-myc expression following exposure to IL-6. The results confirmed that both c-myb and c-myc are downregulated during differentiation and that the downregulation of c-myb precedes that of c-myc (Fig. 5). Forced expression of Gfi-1B inhibited the downregulation of c-myc (Fig. 5, upper panel), suggesting that Gfi-1B functions upstream of c-myc. On the other hand, forced expression of Gfi-1B had no effect on the initial drop of c-myb expression occurring within 3 h (26) but blocked the complete repression of c-myb occurring between 6 and 24 h following exposure to IL-6 (Fig. 5, middle panel). This suggests that the downregulation of c-myb during M1 cell differentiation is a complex process accomplished in two steps that are under the control of different regulatory processes. Gfi-1B downregulation precedes the second but not the first wave of c-myb downregulation. Although these data show that Gfi-1B contributes to the regulation of c-myc and c-myb in the context of myelomonocytic cell differentiation, they do not imply that its role in the regulation of these genes is direct.
|
IL-6 treatment of M1 cells downregulates Gfi-1B and upregulates p21WAF1 with similar kinetics: forced expression of Gfi-1B inhibits IL-6-mediated induction of p21WAF1. Progression through the cell cycle depends on the activity of a set of kinases, the cyclin-dependent kinases, which are regulated by binding to their regulatory subunits, the cyclins (18, 41, 52), and by phosphorylation (33). The cyclin-cyclin-dependent kinase active complexes are also regulated by cyclin-dependent kinase inhibitors, which bind either to the cyclin-dependent kinase or the cyclin component of the complexes or both (22, 53). Upregulation of cyclin-dependent kinase inhibitors induces cell cycle arrest (14). Given that the expression of Gfi-1B prevents G1 arrest, the cyclin-dependent kinase (cdk) inhibitors are good candidate targets for Gfi-1B repression. To address this hypothesis, we probed Northern blots of total-cell RNA from untreated and IL-6-treated M1 cells with Gfi-1B, p27KIP1, p16INK4A, and p21WAF1 probes. Northern blots of total-cell RNA derived from M1/Gfi-1B cell lines were probed in parallel. The results showed that the downregulation of Gfi-1B in IL-6-treated M1 cells is associated with the upregulation of p21WAF1 and that the kinetics of the downregulation of Gfi-1B and the upregulation of p21WAF1 are similar (Fig. 6A, left panels). However, the upregulation of p21WAF1 was abrogated in M1 cells transfected with pcDNA3/Gfi-1B and expressing Gfi-1B constitutively. This is shown in Fig. 6B, which presents a repeat of the experiment shown in Fig. 6A with pcDNA3- or pcDNA3/Gfi-1B-transfected cells. The changes in the expression of Gfi-1B and p21WAF1 at the RNA level paralleled similar changes at the protein level (Fig. 6A and B, right panels).
|
SNAG and Gfi-1BNter, two Gfi-1B mutants defective in
transcriptional repression function, failed to inhibit IL-6-induced G1 arrest and differentiation of M1 cells (Fig. 4). To
determine whether these mutants were also defective in preventing
induction of p21WAF1, we examined the expression
of Gfi-1B and p21WAF1 in Gfi-1BSNAG- and
Gfi-1BNter-transfected M1 cells before and after IL-6 treatment.
The results (Fig. 6C) revealed that overexpression of the mutants
does not inhibit p21WAF1 induction. These
results confirmed that the downregulation of Gfi-1B and the
induction of p21WAF1 are linked and
suggested that Gfi-1B may be a physiological direct repressor of
p21WAF1. Of the other two cyclin-dependent
kinase inhibitors whose expression was examined in these cells,
p16INK4A was undetectable and
p27KIP1 exhibited a pattern of expression that
did not correlate with that of Gfi-1B (data not shown).
Gfi-1B represses the p21WAF1
promoter.
To determine whether the downregulation of
p21WAF1 by Gfi-1B is due to direct
repression of the p21WAF1 promoter, we
cotransfected the p53-deficient mouse embryonic fibroblast cell line
10-1 (23) with a Gfi-1B expression construct and three
progressively deleted p21WAF1 promoter-CAT
reporter constructs: P6 starting at 2514, P7 starting at
1813, and P8 starting at 1369 from the transcription start site
(Fig. 7A) (13). The results
showed that Gfi-1B represses the P6 and P7
p21WAF1 promoter constructs but fails to repress
the P8 promoter construct (Fig. 7B, left panel), suggesting that the
promoter region responsible for the repression maps at 2514 to
1369. Cotransfection of the P7 p21WAF1
reporter construct with the VP16/Gfi-1B chimera (Fig. 3) showed that
the P7 promoter which is repressed by Gfi-1B is activated by the fusion
protein (Fig. 7B, right panel). These results support the hypothesis
that Gfi-1B is a direct repressor of the p21WAF1
promoter.
|
1518 and 1530 (Fig. 7A).
To confirm that Gfi-1B binds this site, we carried out EMSAs with
a synthetic double-stranded oligonucleotide corresponding to this
site as a probe and in vitro-translated Gfi-1B protein. Figure
8Aa, lane 2, shows an autoradiogram of "in vitro"-translated Gfi-1B labeled with
[35S]methionine. The smaller-size bands are likely to
represent the products of alternative translational initiation. Figure
8Ab, lane 2, shows that Gfi-1B binds to and shifts the oligonucleotide corresponding to the putative Gfi-1B binding site in the
p21WAF1 promoter. The binding is specific in
that it is competed by excess unlabeled wild-type but not mutant (AATC
to GGTC) oligonucleotide (lanes 3 and 5 and lanes 4 and 6, respectively). The faster-migrating band could be due to complexes of
the oligonucleotide with the smaller-size Gfi-1B protein products
observed in Fig. 8Aa. EMSAs were also carried out with the same
oligonucleotide derived from the sequence of the
p21WAF1 promoter and nuclear extracts from
IL-6-treated (36 h) and untreated M1 cells (Fig. 8B). The results
showed that nuclear extracts from untreated (lane 2) M1 cells also bind
to the probe, giving rise to one major shifted band which is competed
by excess unlabeled wild-type oligonucleotide (lane 3) but not by its
nonbinding mutant (lane 4) (Fig. 8B). The shift was not detected in
nuclear extracts, however, from IL-6-treated (36 h) M1 cells (lane 7)
in which Gfi-1B is no longer expressed (Fig. 8). An
oligonucleotide derived from the Gfi-1B binding site selection
experiment and a nonbinding mutant of the same oligonucleotide were
also used for competition experiments, and the results were identical
(Fig. 8B, lanes 5 and 6).
|
| |
DISCUSSION |
|---|
|
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
|
|---|
The data presented in this report show that the Gfi-1-related gene Gfi-1B encodes a 329-amino acid protein which is homologous to Gfi-1 in the zinc finger and SNAG repressor domains but which diverges completely from Gfi-1 in the region between the two domains. As expected from these findings, the Gfi-1B protein binds the same DNA sequence as Gfi-1 (66) and functions also as a transcriptional repressor (19, 66). One of the targets of the Gfi-1B repressor is the cyclin-dependent kinase inhibitor p21WAF1.
During IL-6-induced differentiation of the myelomonocytic cell line M1 along the macrophage lineage, Gfi-1B is downregulated to undetectable levels, whereas p21WAF1 is induced. In parallel with these phenomena the M1 cells undergo partial G1 arrest at 48 h from the start of the exposure to IL-6 and they differentiate along the macrophage lineage. Forced expression of Gfi-1B in M1 cells blocks the IL-6-mediated induction of p21WAF1 and inhibits G1 arrest and differentiation. However, Gfi-1B mutants lacking the SNAG domain or the entire amino-terminal region of Gfi-1B fail to inhibit both the induction of p21WAF1 and the cell cycle arrest and differentiation of these cells. These data suggest that IL-6 downregulates Gfi-1B, whose expression in proliferating cells maintains p21WAF1 in a repressed state. Downregulation of Gfi-1B derepresses the p21WAF1 promoter and contributes to the induction of p21WAF1. Expression of p21WAF1 is likely to contribute to the induction of G1 arrest and differentiation in IL-6-treated M1 cells.
If the inhibitory effect of Gfi-1B on the differentiation of M1 cells is due to the repression of p21WAF1, M1 cells defective in p21WAF1 should fail to differentiate in response to IL-6. Preliminary data show that M1 cells overexpressing antisense p21WAF1 indeed failed to undergo G1 arrest and differentiation despite the fact that they downregulated Gfi-1B normally in response to IL-6 (data not shown). These data suggest that p21WAF1 induction may play an important regulatory role in hematopoietic cell differentiation, and they are in agreement with earlier data showing that mice with homozygous inactivation of p21WAF1 exhibit abnormalities in the differentiation of other differentiating cell types such as keratinocytes (40).
M1 cells have been extensively studied as a model of myeloid cell differentiation. Studies with this model system have shown that the differentiation process is marked by changes in the expression of a series of genes (35). Some of these genes are likely to play a regulatory role, whereas others may be important for the expression of the differentiated cell phenotype (2). Two of the regulatory genes, namely c-myb (49) and c-myc (25), behave in a way similar to Gfi-1B during differentiation in that they are both downregulated. Moreover, downregulation of these transcriptional activators is obligatory for differentiation (49) and neither is known to regulate the p21WAF1. Of these, c-myb is downregulated within the first 3 h, while c-myc is downregulated beyond the 6-h time point following exposure to IL-6. As expected from these findings, forced expression of c-myb blocks the downregulation of c-myc and abolishes differentiation (49). Overexpression of c-myc, on the other hand, does not affect c-myb expression and blocks differentiation at an intermediate state (25). The data in this report showed that overexpression of Gfi-1B blocks the downregulation of c-myc and therefore suggest that the downregulation of Gfi-1B not only precedes but is also required for the downregulation of c-myc. The same data revealed unexpectedly that the downregulation of c-myb is a more complex process that takes place in two differentially regulated waves. The first wave, which occurs within the first 3 h following exposure to IL-6, precedes and is independent of the downregulation of Gfi-1B. However, the second wave of c-myb downregulation, which occurs more than 6 h following exposure to IL-6, is blocked by the overexpression of Gfi-1B. These data provide a temporal framework that is required to further explore the potential physiological relationships between these three transcription factors that are sequentially involved in regulating myeloid cell differentiation.
The regulation of the cyclin-dependent kinase inhibitor
p21WAF1 has been the subject of intense study.
Earlier studies had shown that it is induced by the tumor suppressor
gene p53 (12) and that the induction of
p21WAF1 by p53 may be sufficient to explain at
least some of the p53-elicited biological effects.
However, subsequent studies showed that
p21WAF1 may also be induced by
p53-independent mechanisms (11, 27, 28, 39). Transcriptional
regulators other than p53 that contribute to the induction of the
p21WAF1 promoter include MyoD and the adapter
protein p300 (21, 44, 54), the receptor for vitamin D3
(36), the retinoic acid receptor (37), C/EBP
(58), STAT1 (8), SP1 (5), SP3
(43), AP2 (64), homeobox protein Gax
(55), and BRCA1 (56). All the factors regulating
p21WAF1 expression known to date, however, do so
by inducing the activation of its promoter. The data in this report
identify Gfi-1B as a repressor of this promoter, the only such
repressor yet known, and demonstrate that
p21WAF1 expression is regulated by both positive
and negative regulators of transcription. The expression of
p21WAF1 therefore may depend on the balance
between transcriptional inducers and repressors. Since p53 is one of
the main inducers of p21WAF1, Gfi-1B is likely
to compete with p53-elicited biological effects such as cell cycle
arrest and apoptosis. The data presented in this report showed that
Gfi-1B indeed promotes cell cycle progression and therefore support
this hypothesis. We therefore suggest that mutations that inactivate
the p53 gene, which indeed are the most commonly observed
mutations in human cancer (7), and mutations that induce the
expression or enhance the activity of Gfi-1B and perhaps
Gfi-1 may exert overlapping biological effects and may act
synergistically in oncogenesis.
The preceding data showed that Gfi-1B is involved in myelomonocytic cell differentiation. However, the findings showing that Gfi-1B is a direct repressor of p21WAF1 and a potential competitor of p53 suggested that Gfi-1B may also play a role in oncogenesis. This was confirmed recently by experiments showing that Gfi-1B like Gfi-1 is also a target for provirus integration in retrovirus-induced rodent lymphomas. Specifically, Gfi-1B was shown to be involved in Mo-MuLV-induced B-cell lymphomas in Eµ-myc transgenic, pim-1/pim-2 knockout mice (39a). Gfi-1B involvement appears to be specific for these tumors because analysis of 217 DNA samples from 105 Mo-MuLV-induced rat T-cell lymphomas revealed no Gfi-1B involvement (data not shown). The reason for this specificity is that Gfi-1B, like Gfi-1, may cooperate with c-myc (42, 47), although perhaps only in the absence of pim activity.
In summary, the data in this report showed that Gfi-1B, the second known member of the Gfi-1 family of zinc finger proteins, is also a SNAG-domain-containing transcriptional repressor. The Gfi-1B repressor is involved in regulating the process of hematopoietic cell differentiation. In addition, it is involved in lymphoid cell oncogenesis. The differentiation controlling function and perhaps the oncogenic function of Gfi-1B may depend at least partially on the ability of the protein to repress the expression of the cyclin-dependent kinase inhibitor p21WAF1. Although the expression of p21WAF1 can be induced by a multitude of transcriptional activators (5, 8, 21, 36, 37, 43, 44, 54-56, 58, 64), Gfi-1B appears to be its only repressor known to date.
| |
ACKNOWLEDGMENTS |
|---|
We thank H. Mikkers and A. Berns for communicating their data
prior to publication. We also thank M. Flubacher (Fox Chase Cancer
Center [FCCC]) for providing Northern blots for the initial examination of Gfi-1B expression, K. Stamatakis for help with the
generation of the Gfi-1BSNAG and Gfi-1BNter constructs, J. Sherley and Y. Liu (FCCC) for the 10-1 cell line, B. Calabretta and T. Skorski (Kimmel Cancer Center) for the c-myc and
c-myb probes, and P. Bateman for secretarial assistance.
This work was supported by the Public Health Service grant RO1 CA-56110. Additional support was provided by Public Health Service grant CA-06927 and by an appropriation from the Commonwealth of Pennsylvania to the Fox Chase Cancer Center. W.S.E.-D. is an Assistant Investigator of the Howard Hughes Medical Institute. T.-Y.Y. was supported by an L. Greenwald Postdoctoral Fellowship (FCCC). B.T. was a graduate student in the Cell and Molecular Biology program of the University of Pennsylvania School of Medicine.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Fox Chase Cancer Center, 7701 Burholme Avenue, Philadelphia, PA 19111. Phone: (215) 728-3635. Fax: (215) 728-2741. E-mail: tsichlis{at}archimedes.rm.fccc.edu.
Present address: Institute for Cellular Therpeutics, Allegheny
University of the Health Sciences, Philadelphia, PA 19102.
Present address: Dana Farber Cancer Institute, Boston, MA 02115.
§ Present address: Max-Delbrück-Center for Molecular Medicine, 13122 Berlin, Germany.
| |
REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
|
|---|
| 1. |
Anderson, S.,
D. H. Davis,
H. Dahlbäck,
H. Jörnvall, and D. W. Russell.
1989.
Cloning, structure and expression of the mitochondrial cytochrome P-450 sterol 26-hydroxylase, a bile biosynthetic enzyme.
J. Biol. Chem.
264:8222-8229 |
| 2. |
Arnaout, M. A.
1990.
Structure and function of the leukocyte adhesion molecules CD11/CD18.
Blood
75:1037-1050 |
| 3. | Bell, D. W., T. Taguchi, N. A. Jenkins, D. J. Gilbert, N. G. Copeland, C. B. Gilks, P. Zweidler-McKay, H. L. Grimes, P. N. Tsichlis, and J. R. Testa. 1995. Chromosomal localization of a gene, GFI1, encoding a novel zinc finger protein reveals a new syntenic region between man and rodents. Cytogenet. Cell Genet. 70:263-267[Medline]. |
| 4. | Bies, J., B. Hoffman, A. Amanullah, T. Giese, and L. Wolff. 1996. B-Myb prevents growth arrest associated with terminal differentiation of monocytic cells. Oncogene 12:355-363[Medline]. |
| 5. |
Biggs, J. R.,
J. E. Kudlow, and A. S. Kraft.
1996.
The role of the transcription factor Sp1 in regulating the expression of the WAF1/CIP1 gene in U937 leukemic cells.
J. Biol. Chem.
271:901-906 |
| 6. |
Bignon, C.,
D. Daniel, and J. Dijiane.
1993.
-Galactosidase and chloramphenicol acetyltransferase assays in 96-well plates.
BioTechniques
15:243-245.
[Medline] |
| 7. | Bosari, S., and G. Viale. 1995. The clinical significance of p53 aberrations in human tumors. Virchows Arch. 427:229-241[Medline]. |
| 8. | Chin, Y. E., M. Kitagawa, W. C. Su, Z. H. You, Y. Iwamoto, and X. Y. Fu. 1996. Cell growth arrest and induction of cyclin-dependent kinase inhibitor p21 WAF1/CIP1 mediated by STAT1. Science 272:719-722[Abstract]. |
| 9. | Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal. Biochem. 162:156-159[Medline]. |
| 10. | Collins, S. J., S. Tsai, and I. Bernstein. 1996. Retinoic acid receptors in hematopoiesis. Curr. Top. Microbiol. Immunol. 211:7-15[Medline]. |
| 11. | Elbendary, A., A. Berchuck, P. Davis, L. Havrilesky, R. C. Bast, Jr., J. D. Iglehart, and J. R. Marks. 1994. Transforming growth factor beta 1 can induce CIP1/WAF1 expression independent of the p53 pathway in ovarian cancer cells. Cell Growth Differ. 5:1301-1307[Abstract]. |
| 12. | El-Deiry, W. S., T. Tokino, V. E. Velculescu, D. B. Levy, R. Parsons, J. M. Trent, D. Lin, W. E. Mercer, K. W. Kinzler, and B. Vogelstein. 1993. WAF1, a potential mediator of p53 tumor suppression. Cell 75:817-825[Medline]. |
| 13. |
El-Deiry, W. S.,
T. Tokino,
T. Waldman,
J. D. Oliner,
V. E. Velculescu,
M. Burrell,
D. E. Hill,
E. Healy,
J. L. Rees,
S. R. Hamilton,
K. W. Kinzler, and B. Vogelstein.
1995.
Topological control of p21WAF1/CIP1 expression in normal and neoplastic tissues.
Cancer Res.
55:2910-2919 |
| 14. | Elledge, S. J., J. Winston, and J. W. Harper. 1996. A question of balance: the role of cyclin-kinase inhibitors in development and tumorigenesis. Trends Cell Biol. 6:388-392. [Medline] |
| 15. | Gearing, D. P., N. M. Gough, J. A. King, D. J. Hilton, N. A. Nicola, R. J. Simpson, E. C. Nice, A. Kelso, and D. Metcalf. 1987. Molecular cloning and expression of cDNA encoding a murine myeloid leukemia inhibitory factor (LIF). EMBO J. 6:3995-4002[Medline]. |
| 16. |
Gilks, C. B.,
S. E. Bear,
H. L. Grimes, and P. N. Tsichlis.
1993.
Progression of interleukin-2 (IL-2)-dependent rat T cell lymphoma lines to IL-2-independent growth following activation of a gene (Gfi-1) encoding a novel zinc finger protein.
Mol. Cell. Biol.
13:1759-1768 |
| 17. |
Gorman, C. M.,
L. F. Moffat, and B. H. Howard.
1982.
Recombinant genomes which express chloramphenicol acetyltransferase in mammalian cells.
Mol. Cell. Biol.
2:1044-1051 |
| 18. | Graña, X., and E. P. Reddy. 1995. Cell cycle control in mammalian cells: role of cyclins, cyclin-dependent kinases (CDKs), growth suppressor genes and cyclin-dependent kinase inhibitors (CKIs). Oncogene 11:211-219[Medline]. |
| 19. | Grimes, H. L., T. O. Chan, P. A. Zweidler-McKay, B. Tong, and P. N. Tsichlis. 1996. The Gfi-1 proto-oncoprotein contains a novel transcriptional repressor domain, SNAG, and inhibits G1 arrest induced by interleukin-2 withdrawal. Mol. Cell. Biol. 16:6263-6272[Abstract]. |
| 20. |
Grimes, H. L.,
C. B. Gilks,
T. O. Chan,
S. Porter, and P. N. Tsichlis.
1996.
The Gfi-1 proto-oncoprotein represses Bax expression and inhibits T-cell death.
Proc. Natl. Acad. Sci. USA
93:14569-14573 |
| 21. |
Halevy, O.,
B. G. Novitch,
D. B. Spicer,
S. X. Skapek,
J. Rhee,
G. J. Hannon,
D. Beach, and A. B. Lassar.
1995.
Correlation of terminal cell cycle arrest of skeletal muscle with induction of p21 by MyoD.
Science
267:1018-1021 |
| 22. | Harper, J. W., and S. J. Elledge. 1996. Cdk inhibitors in development and cancer. Curr. Opin. Genet. Dev. 6:56-64[Medline]. |
| 23. |
Harvey, D. M., and A. J. Levine.
1991.
p53 alteration is a common event in the spontaneous immortalization of primary BALB/c murine embryo fibroblasts.
Genes Dev.
5:2375-2385 |
| 24. | Hawley, R. G., F. H. L. Lieu, A. Z. C. Fong, and T. S. Hawley. 1994. Versatile retroviral vectors for potential use in gene therapy. Gene Ther. 1:1-11. |
| 25. |
Hoffman-Liebermann, B., and D. A. Liebermann.
1991.
Interleukin-6- and leukemia inhibitory factor-induced terminal differentiation of myeloid leukemia cells is blocked at an intermediate stage by constitutive c-myc.
Mol. Cell. Biol.
11:2375-2381 |
| 26. | Hoffman-Liebermann, B., and D. A. Liebermann. 1991. Suppression of c-myc and c-myb is tightly linked to terminal differentiation induced by IL6 or LIF and not growth inhibition in myeloid leukemia cells. Oncogene 6:903-909[Medline]. |
| 27. | Jiang, H., J. Lin, Z. Z. Su, F. R. Collart, E. Huberman, and P. B. Fisher. 1994. Induction of differentiation in human promyelocytic HL-60 leukemia cells activates p21, WAF1/CIP1, expression in the absence of p53. Oncogene 9:3397-3406[Medline]. |
| 28. | Johnson, M., D. Dimitrov, P. J. Vojta, J. C. Barrett, A. Noda, O. M. Pereira-Smith, and J. R. Smith. 1994. Evidence for a p53-independent pathway for upregulation of SDI1/CIP1/WAF1/p21 RNA in human cells. Mol. Carcinog. 11:59-64[Medline]. |
| 29. | Kelley, K. W., S. Arkins, C. Minshall, Q. Liu, and R. Dantzer. 1996. Growth hormone, growth factors and hematopoiesis. Horm. Res. 45:38-45[Medline]. |
| 30. | Kramer, A., and W. Keller. 1990. Preparation and fractionation of mammalian extracts active in pre-mRNA splicing. Methods Enzymol. 181:3-19[Medline]. |
| 31. | Krystosek, A., and L. Sachs. 1976. Control of lysozyme induction in the differentiation of myeloid leukemic cells. Cell 9:675-684[Medline]. |
| 32. |
Lan, M. S.,
E. K. Russell,
J. Lu,
B. E. Johnson, and A. L. Notkins.
1993.
IA-1, a new marker for neuroendocrine differentiation in human lung cancer cell lines.
Cancer Res.
53:4169-4171 |
| 33. | Lew, D. J., and S. Kornbluth. 1996. Regulatory roles of cyclin-dependent kinase phosphorylation in cell cycle control. Curr. Opin. Cell Biol. 8:795-804[Medline]. |
| 34. | Li, H., P. S. Zeitler, M. T. Valerius, K. Small, and S. S. Potter. 1996. Gsh-1, an orphan Hox gene, is required for normal pituitary development. EMBO J. 15:714-724[Medline]. |
| 35. | Liebermann, D. A., and B. Hoffman. 1994. Differentiation primary response genes and proto-oncogenes as positive and negative regulators of terminal hematopoietic cell differentiation. Stem Cells 12:352-369[Medline]. |
| 36. |
Liu, M.,
M. H. Lee,
M. Cohen,
M. Bommakanti, and L. P. Freedman.
1996.
Transcriptional activation of the Cdk inhibitor p21 by vitamin D3 leads to the induced differentiation of the myelomonocytic cell line U937.
Genes Dev.
10:142-153 |
| 37. |
Liu, M.,
A. Iavarone, and L. P. Freedman.
1996.
Transcriptional activation of the human p21 (WAF1/CIP1) gene by retinoic acid receptor. Correlation with retinoid induction of U937 cell differentiation.
J. Biol. Chem.
271:31723-31728 |
| 38. | Meier, R. W., T. Chen, S. Mathews, G. Niklaus, and A. Tobler. 1992. The differentiation pathway of HL60 cells is a model system for studying the specific regulation of some myeloid genes. Cell Growth Differ. 3:663-669[Abstract]. |
| 39. |
Michieli, P.,
M. Chedid,
D. Lin,
J. H. Pierce,
W. E. Mercer, and D. Givol.
1994.
Induction of WAF1/CIP1 by a p53-independent pathway.
Cancer Res.
54:3391-3395 |
| 39a. | Mikkers, H., and A. Berns. Personal communication. |
| 40. |
Missero, C.,
F. Di Cunto,
H. Kiyokawa,
A. Koff, and G. P. Dotto.
1996.
The absence of p21Cip1/WAF1 alters keratinocyte growth and differentiation and promotes ras-tumor progression.
Genes Dev.
10:3065-3075 |
| 41. | Morgan, D. O. 1995. Principles of CDK regulation. Nature 374:131-134[Medline]. |
| 42. | Orkin, S. H. 1996. Development of hematopoietic system. Curr. Opin. Genet. Dev. 6:597-602[Medline]. |
| 43. |
Prowse, D. M.,
L. Bolgan,
A. Molnar, and G. P. Dotto.
1997.
Involvement of the Sp3 transcription factor in induction of p21Cip1/WAF1 in keratinocyte differentiation.
J. Biol. Chem.
272:1308-1314 |
| 44. | Puri, P. L., M. L. Avantaggiati, C. Balsano, N. Sang, A. Graessmann, A. Giordano, and M. Levrero. 1997. p300 is required for MyoD-dependent cell cycle arrest and muscle-specific gene transcription. EMBO J. 16:369-383[Medline]. |
| 44a. | Ryan, K., I. Hayes, R. J. B. Nibbs, J. W. Baird, B. Tong, P. N. Tsichlis, J. D. Ansell, N. Hole, and G. J. Graham. Submitted for publication. |
| 45. | Sachs, L. 1990. The control of growth and differentiation in normal and leukemic blood cells. Cancer 65:2196-2206[Medline]. |
| 46. |
Sachs, L.
1996.
The control of hematopoiesis and leukemia: from basic biology to the clinic.
Proc. Natl. Acad. Sci. USA
93:4742-4749 |
| 47. | Scheijen, B., J. Jonkers, D. Acton, and A. Berns. 1997. Characterization of pal-1, a common proviral insertion site in murine leukemia virus-induced lymphomas of c-myc and Pim-1 transgenic mice. J. Virol. 71:9-16[Abstract]. |
| 48. |
Schmidt, T.,
M. Zornig,
R. Beneke, and T. Moroy.
1996.
MoMuLV proviral integrations identified by Sup-F selection in tumors from infected myc/pim bitransgenic mice correlate with activation of the gfi-1 gene.
Nucleic Acids Res.
24:2528-2534 |
| 49. |
Selvakumaran, M.,
D. A. Liebermann, and B. Hoffman-Liebermann.
1992.
Deregulated c-myb disrupts interleukin-6- or leukemia inhibitory factor-induced myeloid differentiation prior to c-myc: role in leukemogenesis.
Mol. Cell. Biol.
12:2493-2500 |
| 50. |
Shabo, Y.,
J. Lotem,
M. Rubinstein,
M. Revel,
S. C. Clark,
S. F. Wolf,
R. Kamen, and L. Sachs.
1988.
The myeloid blood cell differentiation-inducing protein MGI-2A is interleukin-6.
Blood
72:2070-2073 |
| 51. |
Sherley, J. L., and T. J. Kelly.
1988.
Regulation of human thymidine kinase during the cell cycle.
J. Biol. Chem.
263:8350-8358 |
| 52. |
Sherr, C. J.
1996.
Cancer cell cycles.
Science
274:1672-1677 |
| 53. |
Sherr, C. J., and J. M. Roberts.
1995.
Inhibitors of mammalian G1 cyclin-dependent kinases.
Genes Dev.
9:1149-1163 |
| 54. |
Skapek, S. X.,
J. Rhee,
D. B. Spicer, and A. B. Lassar.
1995.
Inhibition of myogenic differentiation in proliferating myoblasts by cyclin D1-dependent kinase.
Science
267:1022-1024 |
| 55. |
Smith, R. C.,
D. Branellec,
D. H. Gorski,
K. Guo,
H. Perlman,
J.-F. Dedieu,
C. Pastore,
A. Mahfoudi,
P. Denèfle,
J. M. Isner, and K. Walsh.
1997.
p21CIP1-mediated inhibition of cell proliferation by overexpression of the gax homeodomain gene.
Genes Dev.
11:1674-1689 |
| 56. | Somasundaram, K., H. Zhang, Y.-X. Zeng, Y. Houvras, Y. Peng, H. Zhang, G. S. Wu, J. D. Licht, B. L. Weber, and W. S. El-Deiry. 1997. Arrest of the cell cycle by the tumour-suppressor BRCA1 requires the CDK-inhibitor p21WAF1/CIP1. Nature 389:187-190[Medline]. |
| 57. | Steinman, R. A., B. Hoffman, A. Iro, C. Guillouf, D. A. Liebermann, and M. E. el-Houseini. 1994. Induction of p21 (WAF-1/CIP1) during differentiation. Oncogene 9:3389-3396[Medline]. |
| 58. |
Timchenko, N. A.,
M. Wilde,
M. Nakanishi,
J. R. Smith, and G. J. Darlington.
1996.
CCAAT/enhancer-binding protein (C/EBP ) inhibits cell proliferation through the p21 (WAF-1/CIP-1/SDI-1) protein.
Genes Dev.
10:804-815 |
| 59. | Tong, B. 1997. In Gfi-1B represses p21WAF1 expression and inhibits myeloid cell differentiation. Ph.D. thesis. University of Pennsylvania, Philadelphia. |
| 59a. | Tong, B., N. Copeland, and N. Jenkins. Unpublished data. |
| 60. |
Vasavada, H. A.,
S. Ganguly,
F. J. Germino,
Z. X. Wang, and S. M. Weissman.
1991.
A contingent replication assay for the detection of protein-protein interactions in animal cells.
Proc. Natl. Acad. Sci. USA
88:10686-10690 |
| 61. |
Weeks, D. L., and N. C. Jones.
1983.
E1A control of gene expression is mediated by sequences 5' to the transcriptional starts of the early viral genes.
Mol. Cell. Biol.
3:1222-1234 |
| 62. | Yonish-Rouach, E., D. Resnitzky, J. Lotem, L. Sachs, A. Kimchi, and M. Oren. 1991. Wild-type p53 induces apoptosis of myeloid leukemic cells that is inhibited by interleukin-6. Nature 352:345-347[Medline]. |
| 63. | Zanjani, E. D., G. Almeida-Porada, and A. W. Flake. 1996. The human/sheep xenograft model: a large animal model of human hematopoiesis. Int. J. Hematol. 63:179-192[Medline]. |
| 64. | Zeng, Y. X., K. Somasundaram, and W. S. El-Deiry. 1997. AP2 inhibits cancer cell growth and activates p21WAF1/CIP1 expression. Nat. Genet. 15:78-82[Medline]. |
| 65. | Zhang, D. E., S. Hohaus, M. T. Voso, H. M. Chen, L. T. Smith, C. J. Hetherington, and D. G. Tenen. 1996. Function of PU.1 (Spi-1), C/EBP, and AML1 in early myelopoiesis: regulation of multiple myeloid CSF receptor promoters. Curr. Top. Microbiol. Immunol. 211:137-147[Medline]. |
| 66. | Zweidler-McKay, P. A., H. L. Grimes, M. M. Flubacher, and P. N. Tsichlis. 1996. Gfi-1 encodes a nuclear zinc finger protein that binds DNA and functions as a transcriptional repressor. Mol. Cell. Biol. 16:4024-4034[Abstract]. |
Mol Cell Biol, May 1998, p. 2462-2473, Vol. 18, No. 5
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
This article has been cited by other articles:
-
Holm, R, Knopp, S, Kumar, R, Lee, J, Nesland, J M, Trope, C, Callen, D F
(2008). Expression of ZNF652, a novel zinc finger protein, in vulvar carcinomas and its relation to prognosis. J. Clin. Pathol.
61: 59-63
[Abstract] [Full Text] -
Marteijn, J. A. F., van der Meer, L. T., van Emst, L., van Reijmersdal, S., Wissink, W., de Witte, T., Jansen, J. H., Van der Reijden, B. A.
(2007). Gfi1 ubiquitination and proteasomal degradation is inhibited by the ubiquitin ligase Triad1. Blood
110: 3128-3135
[Abstract] [Full Text] -
De La Luz Sierra, M., Gasperini, P., McCormick, P. J., Zhu, J., Tosato, G.
(2007). Transcription factor Gfi-1 induced by G-CSF is a negative regulator of CXCR4 in myeloid cells. Blood
110: 2276-2285
[Abstract] [Full Text] -
Kuo, Y.-Y., Chang, Z.-F.
(2007). GATA-1 and Gfi-1B Interplay To Regulate Bcl-xL Transcription. Mol. Cell. Biol.
27: 4261-4272
[Abstract] [Full Text] -
Vassen, L., Okayama, T., Moroy, T.
(2007). Gfi1b:green fluorescent protein knock-in mice reveal a dynamic expression pattern of Gfi1b during hematopoiesis that is largely complementary to Gfi1. Blood
109: 2356-2364
[Abstract] [Full Text] -
Dahl, R., Iyer, S. R., Owens, K. S., Cuylear, D. D., Simon, M. C.
(2007). The Transcriptional Repressor GFI-1 Antagonizes PU.1 Activity through Protein-Protein Interaction. J. Biol. Chem.
282: 6473-6483
[Abstract] [Full Text] -
Zhu, J., Jankovic, D., Grinberg, A., Guo, L., Paul, W. E.
(2006). Gfi-1 plays an important role in IL-2-mediated Th2 cell expansion. Proc. Natl. Acad. Sci. USA
103: 18214-18219
[Abstract] [Full Text] -
Acar, M., Jafar-Nejad, H., Giagtzoglou, N., Yallampalli, S., David, G., He, Y., Delidakis, C., Bellen, H. J.
(2006). Senseless physically interacts with proneural proteins and functions as a transcriptional co-activator. Development
133: 1979-1989
[Abstract] [Full Text] -
Duan, Z., Zarebski, A., Montoya-Durango, D., Grimes, H. L., Horwitz, M.
(2005). Gfi1 Coordinates Epigenetic Repression of p21Cip/WAF1 by Recruitment of Histone Lysine Methyltransferase G9a and Histone Deacetylase 1. Mol. Cell. Biol.
25: 10338-10351
[Abstract] [Full Text] -
Huang, D.-Y., Kuo, Y.-Y., Chang, Z.-F.
(2005). GATA-1 mediates auto-regulation of Gfi-1B transcription in K562 cells. Nucleic Acids Res
33: 5331-5342
[Abstract] [Full Text] -
Dwivedi, P. P, Anderson, P. H, Omdahl, J. L, Grimes, H L., Morris, H. A, May, B. K
(2005). Identification of growth factor independent-1 (GFI1) as a repressor of 25-hydroxyvitamin D 1-alpha hydroxylase (CYP27B1) gene expression in human prostate cancer cells. Endocr Relat Cancer
12: 351-365
[Abstract] [Full Text] -
Vassen, L., Fiolka, K., Mahlmann, S., Möröy, T.
(2005). Direct transcriptional repression of the genes encoding the zinc-finger proteins Gfi1b and Gfi1 by Gfi1b. Nucleic Acids Res
33: 987-998
[Abstract] [Full Text] -
Garcon, L., Lacout, C., Svinartchouk, F., Le Couedic, J.-P., Villeval, J.-L., Vainchenker, W., Dumenil, D.
(2005). Gfi-1B plays a critical role in terminal differentiation of normal and transformed erythroid progenitor cells. Blood
105: 1448-1455
[Abstract] [Full Text] -
Jafar-Nejad, H., Bellen, H. J.
(2004). Gfi/Pag-3/Senseless Zinc Finger Proteins: a Unifying Theme?. Mol. Cell. Biol.
24: 8803-8812
[Full Text] -
Ma, X., Bacci, S., Mlynarski, W., Gottardo, L., Soccio, T., Menzaghi, C., Iori, E., Lager, R. A., Shroff, A. R., Gervino, E. V., Nesto, R. W., Johnstone, M. T., Abumrad, N. A., Avogaro, A., Trischitta, V., Doria, A.
(2004). A common haplotype at the CD36 locus is associated with high free fatty acid levels and increased cardiovascular risk in Caucasians. Hum Mol Genet
13: 2197-2205
[Abstract] [Full Text] -
Huang, D.-Y., Kuo, Y.-Y., Lai, J.-S., Suzuki, Y., Sugano, S., Chang, Z.-F.
(2004). GATA-1 and NF-Y cooperate to mediate erythroid-specific transcription of Gfi-1B gene. Nucleic Acids Res
32: 3935-3946
[Abstract] [Full Text] -
Doan, L. L., Porter, S. D., Duan, Z., Flubacher, M. M., Montoya, D., Tsichlis, P. N., Horwitz, M., Gilks, C. B., Grimes, H. L.
(2004). Targeted transcriptional repression of Gfi1 by GFI1 and GFI1B in lymphoid cells. Nucleic Acids Res
32: 2508-2519
[Abstract] [Full Text] -
Jafar-Nejad, H., Acar, M., Nolo, R., Lacin, H., Pan, H., Parkhurst, S. M., Bellen, H. J.
(2003). Senseless acts as a binary switch during sensory organ precursor selection. Genes Dev.
17: 2966-2978
[Abstract] [Full Text] -
Sharina, I. G., Martin, E., Thomas, A., Uray, K. L., Murad, F.
(2003). CCAAT-binding factor regulates expression of the {beta}1 subunit of soluble guanylyl cyclase gene in the BE2 human neuroblastoma cell line. Proc. Natl. Acad. Sci. USA
100: 11523-11528
[Abstract] [Full Text] -
Yu, C.-R., Mahdi, R. M., Ebong, S., Vistica, B. P., Gery, I., Egwuagu, C. E.
(2003). Suppressor of Cytokine Signaling 3 Regulates Proliferation and Activation of T-helper Cells. J. Biol. Chem.
278: 29752-29759
[Abstract] [Full Text] -
Duan, Z., Horwitz, M.
(2003). Targets of the transcriptional repressor oncoprotein Gfi-1. Proc. Natl. Acad. Sci. USA
100: 5932-5937
[Abstract] [Full Text] -
Yucel, R., Karsunky, H., Klein-Hitpass, L., Moroy, T.
(2003). The Transcriptional Repressor Gfi1 Affects Development of Early, Uncommitted c-Kit+ T Cell Progenitors and CD4/CD8 Lineage Decision in the Thymus. JEM
197: 831-844
[Abstract] [Full Text] -
Doan, L. L., Kitay, M. K., Yu, Q., Singer, A., Herblot, S., Hoang, T., Bear, S. E., Morse, H. C. III, Tsichlis, P. N., Grimes, H. L.
(2003). Growth Factor Independence-1B Expression Leads to Defects in T Cell Activation, IL-7 Receptor {alpha} Expression, and T Cell Lineage Commitment. J. Immunol.
170: 2356-2366
[Abstract] [Full Text] -
Wallis, D., Hamblen, M., Zhou, Y., Venken, K. J. T., Schumacher, A., Grimes, H. L., Zoghbi, H. Y., Orkin, S. H., Bellen, H. J.
(2003). The zinc finger transcription factor Gfi1, implicated in lymphomagenesis, is required for inner ear hair cell differentiation and survival. Development
130: 221-232
[Abstract] [Full Text] -
Osawa, M., Yamaguchi, T., Nakamura, Y., Kaneko, S., Onodera, M., Sawada, K.-i., Jegalian, A., Wu, H., Nakauchi, H., Iwama, A.
(2002). Erythroid expansion mediated by the Gfi-1B zinc finger protein: role in normal hematopoiesis. Blood
100: 2769-2777
[Abstract] [Full Text] -
Wu, Q., Kirschmeier, P., Hockenberry, T., Yang, T.-Y., Brassard, D. L., Wang, L., McClanahan, T., Black, S., Rizzi, G., Musco, M. L., Mirza, A., Liu, S.
(2002). Transcriptional Regulation during p21WAF1/CIP1-induced Apoptosis in Human Ovarian Cancer Cells. J. Biol. Chem.
277: 36329-36337
[Abstract] [Full Text] -
Fizazi, K., Martinez, L. A., Sikes, C. R., Johnston, D. A., Stephens, L. C., McDonnell, T. J., Logothetis, C. J., Trapman, J., Pisters, L. L., Ordonez, N. G., Troncoso, P., Navone, N. M.
(2002). The Association of p21(WAF-1/CIP1) with Progression to Androgen-independent Prostate Cancer. Clin. Cancer Res.
8: 775-781
[Abstract] [Full Text] -
Saleque, S., Cameron, S., Orkin, S. H.
(2002). The zinc-finger proto-oncogene Gfi-1b is essential for development of the erythroid and megakaryocytic lineages. Genes Dev.
16: 301-306
[Abstract] [Full Text] -
Cameron, S., Clark, S. G., McDermott, J. B., Aamodt, E., Horvitz, H. R.
(2002). PAG-3, a Zn-finger transcription factor, determines neuroblast fate in C. elegans. Development
129: 1763-1774
[Abstract] [Full Text] -
Sykes, D. B., Kamps, M. P.
(2001). Estrogen-dependent E2a/Pbx1 myeloid cell lines exhibit conditional differentiation that can be arrested by other leukemic oncoproteins. Blood
98: 2308-2318
[Abstract] [Full Text] -
Tateno, M., Fukunishi, Y., Komatsu, S., Okazaki, Y., Kawai, J., Shibata, K., Itoh, M., Muramatsu, M., Held, W. A., Hayashizaki, Y.
(2001). Identification of a Novel Member of the Snail/Gfi-1 Repressor Family, mlt 1, Which Is Methylated and Silenced in Liver Tumors of SV40 T Antigen Transgenic Mice. Cancer Res.
61: 1144-1153
[Abstract] [Full Text] -
Baird, J. W., Ryan, K. M., Hayes, I., Hampson, L., Heyworth, C. M, Clark, A., Wootton, M., Ansell, J. D., Menzel, U., Hole, N., Graham, G. J.
(2001). Differentiating Embryonal Stem Cells Are a Rich Source of Haemopoietic Gene Products and Suggest Erythroid Preconditioning of Primitive Haemopoietic Stem Cells. J. Biol. Chem.
276: 9189-9198
[Abstract] [Full Text] -
Jegalian, A. G., Wu, H.
(2002). Regulation of Socs Gene Expression by the Proto-oncoprotein GFI-1B. TWO ROUTES FOR STAT5 TARGET GENE INDUCTION BY ERYTHROPOIETIN. J. Biol. Chem.
277: 2345-2352
[Abstract] [Full Text]
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Copyright © 2009 by the American Society for Microbiology. For an alternate route to Journals.ASM.org, visit: http://intl-journals.asm.org | More Info»