(Received for publication, March 12, 1997, and in revised form, June 5, 1997)
From the Fels Institute for Cancer Research and Molecular Biology, Temple University School of Medicine, Philadelphia, Pennsylvania 19140
The myb gene family consists of three members, named A-, B-, and c-myb, which encode nuclear proteins that bind to DNA and function as regulators of transcription. Our results show that murine A-myb is a poor transactivator of transcription compared with murine c-myb. Deletion of the COOH-terminal domain of A-Myb, or co-expression with Ets-2 resulted in increased transactivation potential. While ectopic overexpression of c-myb in 32Dcl3 cells results in a block to the ability of these cells to undergo terminal differentiation resulting in indefinite growth in granulocyte-colony-stimulating factor (G-CSF), similar overexpression of A-myb results in growth arrest and concomitant terminal differentiation of 32D cells into granulocytes. Co-expression of A-myb and ets-2 in these cells results in the restoration of the proliferative activity of the cells in G-CSF, but fails to induce a block to G-CSF-induced terminal differentiation. However, overexpression of the COOH-terminal deletion mutant of A-myb results in a block to G-CSF-induced differentiation of 32D cells, suggesting that the distinctive biological phenotypes produced by A-myb and c-myb genes are mediated by their COOH-terminal domains.
The myb gene family currently consists of three members, named A-, B-, and c-myb (1). All the three members of this family code for nuclear proteins that bind DNA in a sequence-specific manner and function as regulators of transcription (2-9). The first one-third of each protein consists of the DNA-binding domain followed by the central portion of the molecule, which seems to mediate the transactivating function of the protein (3, 4). The COOH-terminal end of these proteins contains a third domain, which appears to regulate the transactivating function of these three proteins (3, 4).
c-myb is predominantly expressed in hematopoietic cells and is readily induced upon treatment of these cells with interleukins or mitogens (10, 11). Studies with antisense oligonucleotides demonstrate that expression of the c-myb gene product is essential for the proliferative potential of several myeloid and T-cell lines (12). In addition, studies with hematopoietic cell lines suggest that terminal differentiation of these cells is accompanied by down-regulation of myb gene expression and constitutive expression of c-myb blocks their terminal differentiation (13-22). Homozygous null c-myb mutant mice die in utero due to defects in fetal hepatic hematopoiesis, confirming an essential role for c-myb in hematopoiesis (23).
In contrast to c-myb, little is known about the role of the A-myb and B-myb genes in development. While B-myb seems to be expressed ubiquitously, A-myb is expressed at high levels in testis, germinal centers of spleen, and immature neuronal cells (9, 24). Homozygous null A-myb mutant mice show defects in spermatogenesis and breast development, suggesting that this gene may play an essential role in the development of tissues where it is expressed (25). In addition, A-myb was shown to be expressed in Burkitt's lymphoma cell lines, suggesting that A-myb might be also involved in pre-B-cell development (26). To date, at least two reports indicate that human and chicken A-myb genes are potent transactivators of transcription (7, 8) and based on structural similarities to c-myb, and its apparent transactivating potential, it has been proposed that A-myb might function in an identical manner to that of c-myb in vivo (7, 8). To test this hypothesis, we have examined the relative transactivating potential of murine A-Myb and c-Myb. It was earlier demonstrated that c-Myb co-operates with Ets-2 in transcriptional transactivation of Myb target genes (6). In this report, we examined whether A-myb can similarly co-operate with Ets-2 in transcriptional activation of promoters containing Myb-binding sites. In addition, we have examined the effects of overexpression of A-myb and c-myb on myeloid cell differentiation using the murine myeloid precursor cell line, 32Dcl3. Our results show that c-myb and A-myb differ in their ability to transactivate transcription of reporter genes linked to Myb-responsive promoters but resemble each other in their ability to co-operate with Ets-2. Overexpression of c-myb in 32D cells was found to result in a block to G-CSF1-induced terminal differentiation and accelerated proliferation of these cells, while similar overexpression of A-myb was found to result in their growth arrest. These results suggest that A-myb and c-myb do not perform identical functions in vivo. Our results also suggest that the COOH-terminal domain of A-Myb might confer these distinctive properties to A-Myb.
NIH3T3 cells were cultured in Dulbecco's Modified Eagle medium supplemented with 10% calf serum and 0.5% penicillin/streptomycin (Life Technologies, Inc.) in a humidified incubator maintained at 37 °C circulated with 5% CO2. The murine myeloid progenitor cell line, 32Dcl3 (27-29) was maintained as described earlier supplemented with 10% WEHI3B cell-conditioned medium as a source of IL-3 (30).
PlasmidsConstruction of the reporter plasmid pMIL-luc,
pE-luc-AM, pTA3-luc, and pT81-luc has been described previously (6,
31-33). For expression in NIH3T3 cells, each construct was inserted
into the expression vector pRC/CMV (Invitrogen), which places the
inserts under the control of cytomegalovirus immediate early promoter. RSV-
-Gal plasmid (Invitrogen), which expresses lacZ gene,
was used as an internal standard for transient transfection assays. The
inducible vector pMT-neo, which has the human metallothionein promoter
containing metal-responsive elements (34) and modified from parental
plasmid LK-444 (35), was kindly provided by Dr. Dan Libermann. The
wild-type A-myb and c-myb cDNAs were
subcloned into the pMT-neo vector to express these genes in 32Dcl3
cells in a metal ion-inducible manner. ets-1 and
ets-2 expression vectors were prepared by the insertion of
the two cDNAs (6) into pSG5 vector for SV40-driven expression.
The COOH-terminal truncated mutants of the c-myb and A-myb were constructed using the polymerase chain reaction utilizing primers tagged with NotI and XbaI sites and the polymerase chain reaction product was ligated to pRC/CMV (Invitrogen) and pMT-neo. The inserts were completely sequenced to assure that the polymerase chain reaction reactions did not introduce any mutations in the two genes.
AntiseraTo generate anti-c-Myb antiserum, the part of the c-myb cDNA corresponding to the DNA-binding and transactivation domains (amino acid 1-325) was subcloned into the pDS5-6His vector (Quiaexpress) to produce a fusion protein with 6 histidine residues at the NH2 terminus. The resulting fusion protein was purified by nickel chelate affinity chromatography (Quiaexpress) and used to produce polyclonal antibodies in rabbits.
Transient Transfections and Luciferase AssaysFor
transfection into NIH3T3 cells, cells were seeded into 100-mm dishes at
a density of 1.5-2 × 105 cells/plate. The following
day, DNA was transfected by the calcium phosphate precipitation method
(36). In each transfection, 5 µg of reporter and 5 µg of effector
plasmids were transfected along with 0.5 µg of RSV--Gal plasmid as
an internal standard. Following incubation for 60-70 h, cells were
harvested in 900 µl of reporter lysis buffer (Promega). Luciferase
activity was assayed using a luciferin substrate (Promega) according to
the manufacturer's protocol. Luciferase activities were normalized against the
-galactosidase activity to determine relative luciferase activity, and the activation fold was obtained by setting the value of
the empty vector control as 1.0.
For stable transfection of 32Dcl3 cells, exponentially growing 32Dcl3 cells were electroporated with various plasmid DNAs using a Gene-Pulser (Bio-Rad) at a pulse of 230 V, 960 microfarads. The surviving cells were selected in 500 µg/ml of G418 (Life Technologies, Inc.) for 2-3 weeks. To isolate single cell clones, mass cell cultures were serially diluted in 96-well plates in the presence of G418 and selected for clonal expansion.
Northern Blot AnalysisTotal RNA from each cell line was purified using the Ultra-spec RNA (Biotecx) purification reagent. To purify RNA from zinc-induced cells, the cells were incubated in the presence of 100 µM ZnCl2 for 30 h prior to RNA isolation. Northern blot analysis was performed as described previously (36). To detect the A-myb transcript, an A-myb-specific probe was generated from the 1.35-kbp HindIII-SacI fragment (9). To detect truncated A-myb transcripts, full-length A-myb cDNA (9) was used. To detect c-myb transcripts, a 2.3-kbp cDNA fragment containing the entire stretch of coding sequences was isolated by digestion with BamHI and HindIII and used as a probe.
Western Blot AnalysisTo analyze protein products of the transfected genes, normalized amounts of protein from each cell lysate were separated by SDS-polyacrylamide gel electrophoresis (36), and the separated proteins were transferred to a polyvinylidene difluoride membrane (Millipore) in transfer buffer (10 mM CAPS, 10% methanol, pH 11.0). The filter was blocked with 5% non-fat milk in TTS solution (0.05% Tween 20, 25 mM Tris-HCl, pH 7.4, 150 mM NaCl) for 4 h and incubated with primary antibody in the same buffer for 1 h and washed three times in TTS solution. The secondary antibody reaction was performed by incubating the filters with horseradish peroxidase-conjugated anti-rabbit Ig (Amersham Corp.) and washed in a similar manner as was described for the primary antibody reaction. The Amersham ECL detection system was used for visualization as specified by the manufacturer.
Growth and Differentiation AssaysTo induce granulocytic differentiation, parental or transfected 32D cells were washed twice in IL-3-free medium and plated at a density of 1 × 105 cells/ml in Iscove's modified Dulbecco's medium containing 10% fetal bovine serum and 10% G-CSF (27). The viability and proliferation of the cell cultures were monitored for the indicated days. Morphological analysis of G-CSF-treated cells was performed using an aliquot of cells that was cytospun and stained with May-Grunwald-Giemsa stain. The differentiation state of cells was scored for 12 days at 2-day intervals following the addition of G-CSF to the culture medium. In experiments where metallothionein promoter was used, transcriptional induction of the transgenes was achieved by the addition of 100 µM (final concentration) of ZnCl2 30 h before the addition of G-CSF.
Fig.
1A provides a comparison of
the structure of murine A-Myb and c-Myb proteins. Both these proteins
contain an NH2-terminal DNA-binding domain, a central
transactivation domain, and a carboxyl-terminal negative regulatory
domain. The two proteins exhibit 93, 63, and 62% sequence identities
in the DNA-binding, transactivation, and negative regulatory domains,
respectively (9). As is expected, both proteins have been shown to bind
to the same target sequence (PyrAACGTPur, where Pyr indicates a
pyrimidine and Pur indicates a purine) in DNA (7). Based on the
structural homology and DNA binding properties, several investigators
have suggested that the two genes might possess overlapping biochemical
and biological functions (7, 8, 24, 37). To test this hypothesis, we carried out transcriptional transactivation studies using eukaryotic expression vectors that express full-length murine A-Myb and c-Myb proteins. To avoid problems associated with interspecies differences, all experiments were carried out using the mouse cell lines and mouse
cDNAs. Fig. 1B shows the two reporter plasmids, pMIL-luc and pTA3-luc. The reporter plasmid pMIL was generated by cloning the
naturally occurring Myb-inducible promoter of the mim-1 gene into a luciferase vector. mim-1 promoter was previously
shown to contain three Myb-binding sites (A, B, and
C), of which site A was found to be the high affinity site
(33), and mutations in this site (pE-luc-AM) were found to
drastically reduce Myb-mediated transcriptional transactivation. The
reporter plasmid, pTA3-luc, contains three copies of Myb-binding sites
upstream of a truncated thymidine kinase promoter (31). and pT81-luc,
which lacks Myb-binding sites, was used as a negative control for this
reporter. Fig. 1C illustrates the levels of transactivation
seen with full-length c-myb and A-myb genes when
used with mim-1 promoter. When the reporter gene was placed
under the control of mim-1 promoter, low levels of
transactivation (approximately 3.5 fold) was seen with
c-myb, while no transactivation of the promoter was observed with the A-myb expression vector. p
E-luc-AM, which
contains a mutation in the high-affinity Myb-binding site of the
mim-1 promoter (A-box) showed very little or no
transactivation, when co-transfected with c-myb or
A-myb expression vectors.
To test whether higher transactivation levels can be observed with the synthetic target promoter, we tested the ability of c-myb and A-myb genes to transactivate transcription from the reporter plasmid pTA3. Results shown in Fig. 1D show that while c-myb could transactivate transcription of this reporter by about 10-fold, the A-myb expression vector showed considerably lower transactivation potential (approximately 3-fold), suggesting that murine A-Myb is a weak transactivator, when compared with murine c-Myb. Little or no transactivation was seen with the control vector (pT81-luc) with c-myb and A-myb.
It has been reported previously that the transactivation potential of A-Myb is dose-dependent with a bell-shaped distribution (7). To rule out the possibility that the lower transactivating potential of A-Myb is due to inadequate amounts of DNA used in the transfection studies, we examined the effects of varying amounts of DNA on the transactivation activity of A-Myb. When we varied the amounts of DNA used for transfection in the range of 0.1-10 µg, we observed a dose-dependent increase of activity up to 7 µg of input DNA, which was followed by a drop with increasing concentration of input DNA. A similar dose-response curve was seen with c-myb, which, however, was consistently higher than that of A-myb, suggesting that murine A-myb is indeed a weak transactivator of transcription compared with c-myb (Fig. 1E)
We had previously isolated an alternatively spliced form of A-myb (see A-Myb-AS in Fig. 1A), which codes for a protein that has an internal deletion of 60 amino acids in COOH terminus (9). Because this deletion occurs in the negative regulatory domain, it is conceivable that the protein encoded by this alternatively spliced mRNA exhibits higher transactivation potential than that of full-length A-myb. To test this possibility, we carried out transcriptional transactivation studies using the cDNA that codes for this alternatively spliced form. The results presented in Fig. 1F show that the alternatively spliced form of A-Myb does not significantly differ from the wild-type form, suggesting that this internal deletion does not affect the transactivation potential of the A-Myb protein.
Deletion of the COOH-terminal Negative Regulatory Domain Enhances the Transactivation Potential of Murine A-mybIt has been shown
previously that deletion of COOH-terminal sequences within c-Myb
results in a substantial increase in the transactivating potential of
the truncated protein (3, 4, 6, 38). To determine whether a similar
phenomenon is observed with murine A-myb, we carried out
transfection studies with the truncated forms of A-myb and
c-myb, where the 3 ends of the two genes which encode the
negative regulatory domains have been deleted. The results of these
studies show that deletion of COOH-terminal sequences from both A-Myb
and c-Myb markedly enhance their transactivation potential (Fig.
2A). These results suggest
that like with c-Myb, the COOH-terminal domain of A-Myb acts as a
negative regulatory element and that A-myb can function as a
strong transactivator under conditions that relieve the negative
regulatory effect of the COOH-terminal domain. This is in agreement
with the observations made with human A-myb (37).
A-myb Co-operates with ets-2 in Transcriptional Transactivation of Target Promoters
We had earlier demonstrated that c-Myb and Ets-2 co-operate with each other in transcriptional transactivation of promoters containing Myb-binding sites (6). To test whether the A-myb gene can similarly cooperate with ets-2, the expression plasmid containing A-myb was co-transfected with expression plasmids encoding ets-1 or ets-2 into NIH3T3 cells. As positive controls, identical experiments were carried out with c-myb expression vectors. The two myb genes were expressed under the control of the CMV promoter, while ets-1 or ets-2 genes were driven by the SV40 promoter. This experiment was designed to minimize any promoter interference that might occur when two different constructs are expressed under the control of the same promoter. pTA3-luc was used in this assay, since both c-myb and A-myb genes showed higher transactivation activity with this reporter. As shown in Fig. 2B, co-transfection of the c-myb and ets-2 expression plasmids resulted in approximately 3-fold increase in transactivation as compared with the transactivation levels seen with c-myb alone. However, this increase in transactivation was not observed when the c-myb expression vector was co-transfected with ets-1 expression plasmid, confirming our earlier observation that only ets-2 can mediate this co-operativity (6). We next tested the ability of A-myb to cooperate with ets-1 or ets-2 using the same methods. As presented in Fig. 2B, the transactivation potential of full-length A-Myb was markedly increased (8-fold) when co-transfected with ets-2. The level of co-operativity was considerably higher than that seen with c-Myb, suggesting that A-Myb has a greater ability to co-operate with Ets-2 compared with c-Myb. On the other hand, co-transfection of A-myb and ets-1 did not increase the transactivation potential of A-Myb, suggesting that A-Myb, like c-Myb, cannot cooperate with Ets-1.
A-myb and c-myb Exert Distinctive Biological Effects when Constitutively Expressed in Myeloid Precursor CellsSince A-Myb
and c-Myb proteins share extensive sequence homology and bind to
identical DNA sequence elements, it had been proposed that the two
genes might exert a similar, if not identical, overlapping biological
functions in vivo (7, 8). We had reported earlier a
biological assay for v-myb and c-myb using the
myeloid cell line 32Dcl3 (16, 22). These cells, derived from normal
mouse bone marrow, have been found to be strictly dependent on IL-3 for
growth and undergo terminal differentiation when placed in an IL-3-free
medium containing G-CSF. We had shown previously that overexpression of
v-myb or c-myb in 32Dcl3 cells results in a block
to their ability to terminally differentiate into granulocytes in the
presence of G-CSF (16, 21, 22). To determine whether A-myb
can exert a similar influence during granulocytic differentiation of
32Dcl3 cells, we constructed inducible expression vectors where the
A-myb and c-myb genes were placed under the
control of the human metallothionein promoter. Following the
construction of these vectors, the plasmid DNAs encoding the A-myb and c-myb genes were transfected into
32Dcl3 cells by electroporation. As a negative control, empty vector
DNA was similarly introduced into 32Dcl3 cells. Following selection in
G418, mass cultures as well as single cell clones were established from
each stable transfection. The derived cell lines were tested for the
expression of each transgene in the presence and absence of
Zn2+, which acts as an inducer of transcription from the
metallothionein promoter. The profiles of RNA induction in these cell
lines are shown in Figs. 3A
and 4A. As can be seen in Fig. 3A, 32D cells transfected with the empty vector showed no hybridization with A-myb probe, either in the presence or absence of
Zn2+. On the other hand, mass cultures (32DpMT/A-myb) as
well as three single cell clones (32DpMT/A4, -5, and -6) transfected
with the A-myb expression vector showed low levels of
expression of A-myb transcripts in the absence of
Zn2+, with approximately 10-fold elevation in the
transcription of A-myb transgene in the presence of
Zn2+. When we analyzed the same cell lines for A-Myb
protein expression (Fig. 3B), we did not detect any A-Myb
protein in empty vector-transfected cells, while very low levels of
A-Myb protein was seen in cells transfected with pMT/A-myb but grown in
the absence of Zn2+. However, considerable elevation of
A-Myb protein levels was seen in these cells upon treatment with
Zn2+, which is in agreement with RNA expression data.
Incubation of 32DpMT/A-myb cell line in G-CSF did not result in a
decrease of A-myb transcripts, suggesting that G-CSF does
not down-regulate the expression of the transgene (Fig.
3C).
A similar result was obtained with cells transfected with the
c-myb expression vector, the results of which are shown in
Fig. 4. 32Dcl3 cells transfected with
empty vector DNA (32DpMT neo) showed the presence of a 3.4 kb
endogenous c-myb band in the presence and absence of
Zn2+. In mass cultures (32DpMT/c-myb) as well as single
cell clones (32DpMT/cl3 and -4) transfected with c-myb
expression vectors, low levels of transgene expression were found to
occur, which is seen as a 2.3-kb transcript in the absence of
Zn2+. The smaller size of the transgenic transcript is due
to the absence of 3-untranslated sequence, which was deleted during the construction of the expression plasmid. In the presence of Zn2+, the levels of the 2.3-kb transcript were elevated by
approximately 5-10-fold (Fig. 4A). Interestingly, the
endogenous levels of c-myb RNA were found to be
down-regulated upon the addition of Zn2+, showing an
inverse correlation between transgene expression and endogenous
c-myb RNA expression. Such an alteration of endogenous myb RNA level was not observed in empty vector transfected
cell lines, suggesting that this is not an effect of addition of
ZnCl2 to the culture medium and that autoregulatory
mechanisms function to maintain a constant amount of c-myb
transcript in the cell (39). In agreement with the RNA expression
results, we did not detect a significant increase in the levels of
c-Myb protein upon the addition of Zn2+. To definitively
demonstrate expression of c-Myb protein from the transgene, we compared
the c-Myb protein levels following incubation of 32D cells in the
presence of G-CSF for 12 days. It was shown previously that, in 32Dcl3
cells, the endogenous levels of c-myb transcript and protein
remain relatively high until the 8th day of G-CSF treatment followed by
a down-regulation of RNA and protein, such that they become
undetectable by day 10 of G-CSF treatment (16, 21). Taking advantage of
this observation, we analyzed the level of c-Myb protein on the 12th
day of G-CSF treatment in 32DpMT/c-myb-transfected cells to determine
the levels of c-Myb transgenic protein expressed in the absence of the
endogenous gene product. As shown in Fig. 4B, on the 12th
day of G-CSF treatment, the empty vector-transfected cells were found
to express very little or no c-Myb protein (Fig. 4B, lane 5 and 6). On the other hand, in the pMT/c-myb-transfected
cells, high levels of c-Myb protein could be induced by
Zn2+ (Fig. 4B, lane 7 and 8).
Following the verification of the induction of the transgene, we tested
the effects of overexpression of A-myb and c-myb
on G-CSF-induced terminal differentiation of 32D cells. The results of
these experiments are shown in Fig. 5 and
Table I. 32Dcl3 cells transfected with
the empty vector undergo several rounds of cell division followed by
growth arrest around day 8 of G-CSF treatment in the absence or
presence of Zn2+ (Fig. 5A). On the other hand,
cells transfected with the c-myb expression vector showed a
higher proliferative potential, even in the absence of Zn2+
induction (Fig. 5B). This appears to be due to the
"leaky" expression of low levels of c-myb from the pMT
vector used. However, the proliferation rate of these cells was
dramatically higher in the presence of Zn2+ than in the
absence, suggesting that a higher level of c-myb expression
was responsible for the higher rate of cell proliferation in the
presence of G-CSF (Fig. 5B). In contrast to cells
transfected with c-myb, 32D cells overexpressing
A-myb did not show any increase in the rate of
proliferation. In the absence of Zn2+, the cells
transfected with A-myb expression vectors behaved in a
manner similar to mock-transfected cells, where the cells underwent
several rounds of division followed by growth arrest. On the other
hand, the induction of high levels of A-myb expression in
these cells by the addition of Zn2+ resulted in profound
growth suppression (Fig. 5C), with a decrease in the number
of viable cells during the 10-day course of G-CSF treatment (data not
shown). Levels of A-myb expression remained constant through
the entire period of incubation in G-CSF (Fig. 3C),
suggesting that the observed growth arrest is not a result of shut off
of A-myb transgene expression.
|
Morphological analysis of the cells treated with G-CSF is presented in
Fig. 6. Cells transfected with empty
vector plasmid, when treated with G-CSF, undergo terminal
differentiation into granulocytes by day 10. Similarly, in the absence
of Zn2+, a portion of the cells transfected with
c-myb terminally differentiated into granulocytes by day 10. However, the number of granulocytes were less than that observed with
the mock-transfected cells, presumably due to low level expression of
c-myb from the metallothionein promoter. These cells were
found to undergo growth arrest in an unsynchronized manner and
gradually differentiate into granulocytes by day 15-16 (data not
shown). In the presence of Zn2+, where high levels of
transgene expression were achieved, these cells failed to undergo
terminal differentiation and continued to proliferate indefinitely in
G-CSF containing media as myelocytes/promyelocytes. In contrast to
c-myb transfected cells, the cells transfected with
A-myb expression vector terminally differentiated into
granulocytes in the absence or presence of Zn2+, suggesting
that unlike c-Myb, A-Myb is incapable of blocking G-CSF-induced
terminal differentiation of 32D cells. From these results, we conclude
that ectopic overexpression of c-myb in 32Dcl3 cells results
in a block to G-CSF-induced terminal differentiation with a concomitant
induction of proliferation, while similar overexpression of
A-myb results in an opposite effect leading to a block to
proliferation without affecting G-CSF-induced terminal
differentiation.
Effect of A-Myb and Ets-2 Co-expression on 32D Cell Differentiation
The observation that the transactivating function of A-Myb is highly enhanced in the presence of Ets-2 raised the possibility that A-Myb might mimic the biological activity of c-Myb in the presence of Ets-2, if the weak transactivating activity of A-myb alone is responsible for its inability to induce proliferation of 32Dcl3 cells in the presence of G-CSF. Since the results presented above show that the transactivation potential of A-myb can be considerably enhanced when co-expressed with ets-2, it was of interest to see whether co-expression of ets-2 along with A-myb in 32Dcl3 cells would result in a phenotype that resembles the one produced by c-myb overexpression.
To overexpress Ets-2, an expression plasmid was prepared where the
ets-2 gene was placed under the control of the SV40 promoter (pSG5) along with the puromycin resistance gene, which was placed under
the control of the PGK-1 promoter. This expression vector was
transfected into 32Dcl3 cells, which overexpress A-myb under the control of metallothionein promoter (pMT-neo). As negative controls, empty vectors pSG5 and pMT-neo were similarly electroporated into cells. Following selection of cells in the presence of neomycin and puromycin, the expression of A-myb and ets-2
in these cells was determined by Northern blot analysis. As shown in
Fig. 7A (lane 1),
ets-2 transcripts were undetectable in the 32Dcl3 cell line
transfected with empty vector but were readily detectable in cell lines
that were transfected with pSG5-ets/puro vector (Fig. 7A, lanes
2 and 4). Each cell line was then induced to
differentiate by the addition of G-CSF, and their proliferation rate
and differentiation potential were monitored by cell counting and
morphological analysis. As shown in Fig. 7B, 32Dcl3 cells
transfected with ets-2 expression vector alone in the
absence of A-myb did not show an appreciable increase in the
growth rate compared with control cells that neither expressed
A-myb or ets-2. On the other hand, growth of the
32Dcl3 cell line overexpressing A-myb alone was almost
completely blocked in the presence of G-CSF. However, when the cell
lines expressing both A-myb and ets-2 were
treated with G-CSF, a remarkable increase in the growth of the cells
was observed in the presence of G-CSF (Fig. 7C). In
addition, cell viability was also maintained at a higher level in
ets-2 co-expressing cell line (data not shown). These
results show that A-myb, when co-expressed along with
ets-2, can support the growth of 32Dcl3 cells in the
presence of G-CSF. To determine whether co-expression of
A-myb along with ets-2 resulted in a block to the
ability of 32Dcl3 cells to terminally differentiate into granulocytes,
morphological analysis of cell lines transfected with ets-2
alone, A-myb alone, as well as A-myb along with
ets-2 was carried out. The results of this experiment are
shown in Fig. 7D. These results show that despite their
increased growth rate, the differentiation of 32Dcl3 cells
co-expressing A-myb and ets-2 was not affected.
These results show that co-expression of A-myb along with
Ets-2, while resulting in increased transactivation of the A-Myb
protein, fails to mimic the phenotypic effect produced by c-Myb.
Effect of COOH-terminal Truncation of A-Myb on 32D Cell Differentiation
Since the transactivation potential of A-Myb is
dramatically enhanced by COOH-terminal truncations, we examined the
effects of overexpression of this mutant in 32Dcl3 cells (Fig.
8). For this, we constructed inducible
expression vectors where the truncated A-myb
(tA-myb) gene was placed under the control of the human metallothionein promoter. Following selection in G418, the derived cell
lines were tested for the expression of the transgene in the presence
and absence of Zn2+. Fig. 8A shows the RNA and
protein expression profiles of truncated A-myb in these
transfectants. Interestingly, the expression levels of tA-Myb were very
high even in the absence of Zn2+, which appears to be due
to leaky expression of the transgene from the metallothionein
expression vector.
We next tested the effects of overexpression of tA-myb on G-CSF-induced terminal differentiation of 32D cells. 32Dcl3 cells transfected with the tA-myb expression vector showed a high proliferation potential (Fig. 8B), which is in sharp contrast to cells transfected with full-length A-myb expression vectors. Because of the leaky expression of tA-Myb, addition of Zn2+ did not make a difference to the phenotype observed. Morphological analysis of the cells treated with G-CSF (Fig. 8C) showed that differentiation of these cells is arrested at the myelocytic stage, a phenotype that is similar to that seen with c-myb. From these results, we conclude that the DNA-binding and transactivation domains of A-Myb, in the absence of its COOH-terminal negative regulatory domain can mimic the biological effects of c-Myb. However, full-length A-Myb cannot mimic the biological effects of c-Myb, suggesting that the COOH-terminal domain of A-Myb dictates the biological phenotype produced by this gene.
In this paper, we have described the transactivating potential of murine A-Myb and compared this biochemical activity with that of c-Myb. Our results show that murine A-Myb is a very weak transactivator of transcription compared with that of c-Myb. However, the deletion of the COOH-terminal regulatory domain of A-Myb seemed to restore the full transactivating potential of A-Myb, suggesting that the COOH-terminal domain of this protein exerts a strong negative regulatory effect on this protein. Our results also show that this negative regulatory effect of the COOH-terminal domain could be compensated by Ets-2, which appears to co-operate with A-Myb in transactivation of reporter genes containing Myb-binding sites. Earlier reports with human A-myb (7, 37) had indicated that both A-myb and c-myb gene possess comparable transactivating activity. A similar observation was made with chicken A-myb (8). The reason for this difference is unclear. It is possible that the A-myb gene derived from different species exhibits different transactivational activities. Alternatively, these transactivation assays for human and chicken A-myb were conducted in hematopoietic cell lines, which often express ets-2. Since our results show that co-expression of ets-2 with A-myb results in high transactivational activities, the differences seen by different investigators could be due to the nature of co-operating factors that are expressed in different cell lines.
It is now well established that c-myb is essential for the proliferative potential of several myeloid and T-cell lines (12, 40, 41). In addition, several lines of evidence suggest that hematopoietic cell differentiation is accompanied by down-regulation of c-myb gene expression (10, 11, 42, 43), and constitutive overexpression of c-myb blocks cytokine-induced terminal differentiation of hematopoietic cells (17-22). To test whether A-Myb can function in a manner similar to that of c-Myb in a biological system, we expressed A-myb and c-myb genes in the myeloid precursor cell line 32Dcl3 and examined their effects on the ability of this cell line to undergo terminal differentiation in the presence of G-CSF. Our results clearly show that while expression of c-myb in this cell line results in a block to the ability of these cells to undergo terminal differentiation in the presence of G-CSF, the expression of A-myb failed to bring about this phenotypic effect. In addition, expression of c-myb appears to result in an increased proliferative potential of this cell line in G-CSF, while expression of A-myb alone results in a complete block to the ability of this cell line to proliferate in the presence of G-CSF. The observed inhibitory effect of A-Myb could be attributed to the possibility that A-Myb, by virtue of a highly related DNA-binding domain, could occupy c-Myb binding sites on DNA and act as a competitor to these sites. The inability of A-Myb to bring about transactivation of these c-Myb target genes could bring about the observed growth arrest.
Our observation that the transactivation potential of A-Myb is considerably elevated in the presence of Ets-2 allowed us to test whether A-Myb can mimic the biological effects of c-Myb under conditions where its transactivation potential is enhanced to levels exhibited by c-Myb. Our results show that A-Myb-Ets-2 cooperation results in the restoration of cell proliferation to 32Dcl3 cells incubated in the presence of G-CSF. However, the increase in growth of the cells was not accompanied by an arrest to differentiation process as was observed with c-Myb expression. These results suggest that the cooperation between Ets-2 and A-Myb, while being able to restore its transactivation function, failed to produce the phenotype caused by c-Myb.
Since deletions in the COOH-terminal domain of A-Myb also enhance its
ability to transactivate transcription, we studied the effect of
ectopic overexpression of this mutant on granulocytic differentiation
of 32Dcl3 cells. Our results show that this mutant, tA-myb,
was very effective in promoting proliferation of 32Dcl3 cells in G-CSF
and like c-myb blocked G-CSF-induced differentiation of 32D
cells. These results suggest that the COOH-terminal domain of A-Myb
plays a critical role in the biological phenotype produced by A-Myb and
its deletion allows this protein mimic the function of c-Myb. This was
an unexpected result because of the belief that A-Myb and c-Myb may
both act by similar, if not identical, mechanisms (7, 8). If this were
not to be the case, as suggested by our results, one need to find an
explanation for the opposing effects of A-Myb and c-Myb on 32Dcl3 cell
proliferation and differentiation programs. It is now established that
c-Myb and A-Myb function effectively in the presence of appropriate
co-operating factors, which interact with the two proteins and form an
enhancer complex (6, 44-46). We propose that the nature of
transcription factors that interact with A-Myb or c-Myb is determined
by their COOH-terminal domains, which dictate the nature of the
enhancer complex formed between c-Myb and A-Myb proteins and other
co-operating factors (Fig. 9). In the
absence of any co-operating factors, it is expected that these two
proteins assume an inactive state via an intramolecular conformation
such as the one suggested recently for c-Myb (47). However, following
post-translational modifications, which seem to activate the
transactivating potential of these proteins (48, 49), c-Myb and A-Myb
assume conformations that allow their interaction with discrete sets of
transcription factors, which specify the nature of target genes that
are transactivated by A-Myb and c-Myb. We would propose that the
COOH-terminal domains of the two proteins play an active role in
dictating the nature of factors that interact with each other. It is
likely that some of these factors such as Ets-2 might be common to both
c-Myb and A-Myb, while others (depicted as 1 and
2 in Fig. 9) might be unique to the individual Myb proteins.
This combination of interacting factors is likely to dictate the nature
of target genes that are transactivated by individual members of the
Myb family of proteins. It is possible that c-Myb and A-Myb have some
common targets and some specific targets, which dictate the final
biological effects produced by these individual proteins. It is
conceivable that the COOH-terminal domain of c-Myb allows the
interaction of c-Myb with a defined set of nuclear factors that
activate transcription of a group of target genes that promote
proliferation and block terminal differentiation of myeloid precursor
cells. On the other hand A-Myb, whose function appears to be restricted
primarily to germ cells (9, 24, 25), might transactivate transcription
of a different set of genes by virtue of its ability to interact with a
distinctive set of nuclear factors. This model predicts that
c-myb and A-myb cannot totally compensate for the
biological function of each other. In myeloid cells such as 32Dcl3, it
is conceivable that co-factors that relieve the negative regulation of
c-Myb exist but not for A-myb. Such factors for A-Myb are likely to be
expressed in cell types such as male germ cells, where A-Myb has a well
defined function (25). In the presence of Ets-2, which can interact
with A-Myb, it is possible that the A-Myb protein undergoes a
conformational change, that allows it to form an enhancer complex that
can transactivate transcription of a few but not all of the target
genes of c-Myb. On the other hand, truncation of A-Myb might relieve
the steric inhibitory effects, resulting in the indiscriminate
interaction of the truncated A-Myb protein with co-operating factors
that interact with both c-Myb or A-Myb. Several lines of study suggest
that truncation of c-Myb at the COOH-terminal region is associated with
enhanced transforming activity (50-54), and it is conceivable that
this may also be true for A-Myb. It is at present unclear whether the
COOH-terminal domains of A-Myb and c-Myb regulate the nature of
enhancer complex formed by participating in protein-protein
interactions or solely through steric effect. Studies aimed at studying
the biological effects of A-Myb truncation in vivo and
identification of nuclear factors that interact with A-Myb and c-Myb
and co-operate to bring about the transcriptional transactivation of
their target genes are likely to shed further insight into the
mechanism of action of this gene family.