(Received for publication, October 2, 1995; and in revised form, December 4, 1995)
From the
The c-myc gene encodes a sequence-specific DNA binding protein that activates transcription of cellular genes. Transcription activation by Myc proteins is regulated by phosphorylation of serine and threonine residues within the transactivation domain and by complex formation with the retinoblastoma-related protein p107. In Burkitt's lymphoma, missense mutations within the c-Myc transactivation domain have been found with high frequency. It has been reported that mutant c-Myc proteins derived from Burkitt's lymphoma cell lines are resistant to inhibition by p107, thus providing a rationale for the increased oncogenic activity of these mutant c-Myc proteins. It has been suggested that these mutant c-Myc proteins resist down-modulation by p107 because they lack cyclin A-cdk2-dependent phosphorylation. Here, we have examined three different Burkitt's lymphoma mutant c-Myc proteins found in primary Burkitt's lymphomas and one mutant c-Myc protein detected in a Burkitt's lymphoma cell line. All four have an unaltered ability to activate transcription and are sensitive to inhibition of transactivation by p107. Furthermore, we provide evidence that down-modulation of c-Myc transactivation by p107 does not require phosphorylation of the c-Myc transactivation domain by cyclin A-cdk2. Our data indicate that escape from p107-induced suppression is not a general consequence of all Burkitt's lymphoma-associated c-Myc mutations, suggesting that other mechanisms exist to deregulate c-Myc function.
The proto-oncogene c-myc encodes a short-lived nuclear phosphoprotein with important roles in cellular proliferation, differentiation, neoplasia, and apoptotic cell death (for review, see Lüscher and Eisenman(1990) and Marcu et al.(1992)). A rapid increase in c-myc expression is observed when quiescent cells are stimulated to re-enter the cell cycle by growth factor stimulation (Kelly et al., 1983). In continuously proliferating cells, however, c-myc mRNA and protein levels are invariant throughout the cell cycle (Hann et al., 1985; Thompson et al., 1986). Insight into the function of Myc proteins came from the identification of two motifs in the carboxyl terminus of Myc proteins that are present in several transcription factors: the basic-helix-loop-helix (bHLH) motif and the leucine zipper (Zip). c-Myc forms a heterodimer through its bHLH-Zip domain with the Max protein (Blackwood and Eisenman, 1991), and a specific DNA binding site (CACGTG) has been identified for the complex (Blackwell et al., 1990; Blackwood and Eisenman, 1991; Blackwood et al., 1992; Halazonetis and Kandil, 1991; Prendergast and Ziff, 1991). A strong and highly conserved transcriptional activation domain is located within the amino terminus of Myc proteins (Kato et al., 1990). Importantly, both the transactivation domain and the DNA binding domain are required for transformation (Stone et al., 1987). In addition to specific transcriptional activation, repression by c-Myc has been described for several genes including c-myc itself, the neu proto-oncogene, and the cyclin D1 gene (Penn et al., 1990a; Philipp et al., 1994; Suen and Hung, 1991). Together, these data indicate that Myc proteins are transcription factors that affect cellular physiology by altering the expression of key cellular genes, the altered expression which is ultimately responsible for the myc-induced phenotype.
The activity of Myc proteins is tightly regulated by several independent mechanisms. During the process of cellular differentiation, Myc is replaced by Mad or Mxi in the Max complex, generating novel heterodimers that suppress transcription by interacting with the Sin3 repressor (reviewed by Bernards(1995)). In addition, the amino-terminal transactivation domain is regulated in at least two different ways. Phosphorylation of threonine 58 and serine 62 within the transactivation domain has been shown to occur in a cell cycle-regulated fashion (Lutterbach and Hann, 1994), and mutation of these phosphorylation sites affects transactivation and transformation by c-myc (Albert et al., 1994; Gupta et al., 1993; Henriksson et al., 1993; Pulverer et al., 1994; Seth et al., 1991). In addition, the transactivation domain of c-Myc can form a specific complex with the retinoblastoma-related protein p107, resulting in inhibition of c-Myc transactivation (Beijersbergen et al., 1994; Gu et al., 1994).
Activation of the
proto-oncogene c-myc by gene amplification, proviral
insertions, as well as chromosomal translocation involving the
c-myc locus has been described in a number of human tumors.
The translocation of the c-myc gene on chromosome 8q24 to
immunoglobulin gene loci on chromosome 14q32, 22q11, or 2p12 is
considered to be a central molecular event in the pathogenesis of
Burkitt's lymphoma (BL) ()(Dalla-Favera et
al., 1982). Variability in the breakpoint positions distinguish
between the subtypes endemic and sporadic (Pelicci et al.,
1986). The human c-myc gene is composed of three exons, of
which the first is noncoding. Sporadic BLs typically possess
breakpoints in the first exon or intron of the c-myc gene,
whereas the endemic cases usually have the chromosome 8 breakpoints far
5` to the c-myc gene. A putative repressor binding site has
been identified at the 5`-end of the first exon of c-myc (Siebenlist et al., 1984). Translocations that separate
this exon from the rest of the gene as well as accumulated mutations
within this region could result in a release of the c-myc gene
from the action of the repressor. Exon 1 mutations have also been found
to abrogate the transcriptional attenuation that occurs at the 3`-end
of exon 1 (Bentley and Groudine, 1986a, 1986b; Cesarman et
al., 1987). Within the first intron of the c-myc gene, a
20-base pair region has been identified as the binding site of a
nuclear protein named MIF. This interaction was abrogated by point
mutations present in a BL cell line (Zajac-Kaye et al., 1988).
Mutations in the same region have also been described for other BL cell
lines, supporting the idea that the MIF protein may be an important
factor for control of c-myc expression.
Apart from mutations that affect c-myc expression, recently a number of endemic and sporadic BL cell lines and some primary tumors have been reported to have mutations within the protein-encoding exons 2 and 3 of c-myc (Albert et al., 1994; Bhatia et al., 1993; Yano et al., 1993; Clark et al., 1994; Murphy et al., 1986; Rabbitts et al., 1983, 1984; Showe et al., 1985). In some cases, it has been shown that these mutations are present before the chromosomal translocation takes place, suggesting that mutations within the protein-encoding region of c-myc are an early event in lymphomagenesis (Bhatia et al., 1993). This suggests that the presence of the mutation is not neutral with respect to Myc function but rather that it confers a growth advantage onto the BL tumor cells. This is supported by the finding of several groups that BL-derived mutant c-myc alleles have increased transforming activity in vitro (Frykberg et al., 1987; Henriksson et al., 1993; Hoang et al., 1995).
It has recently been reported that BL-derived mutant c-Myc proteins are resistant to p107-mediated suppression of transactivation (Gu et al., 1994; Hoang et al., 1995). Surprisingly, these mutant c-Myc proteins had a wild type ability to bind p107 (Hoang et al., 1995). It has been suggested that BL-derived mutant c-Myc alleles lack phosphorylation of threonine 58, the phosphorylation of which is dependent on prior phosphorylation of serine 62 by a p107-cyclin A-cdk2 complex. Thus, it has been proposed that in normal cells cyclin A-cdk2 is recruited to the c-Myc transactivation domain by p107, causing it to phosphorylate serine 62. After this has occurred, additional phosphorylation on threonine 58 is possible, leading to down-modulation of c-Myc transactivation (Hoang et al., 1995).
In the present report, we have studied three different BL-derived c-myc point mutants, each described to be the only alteration in the c-myc coding region of the corresponding primary tumor, and one BL-derived c-myc point mutant detected in a cell line. The four mutant c-Myc proteins were analyzed for their ability to transactivate transcription both as GAL4 fusion protein as well as a full-length protein. In contrast to other reports, we find no significant effect of these mutations on c-Myc transactivation and sensitivity to p107 suppression.
Figure 1: Frequency of c-Myc missense mutations in primary Burkitt's lymphoma and in Burkitt's lymphoma cell lines. The numbers above the bars represent amino acid numbers.
To study transactivation by the mutant c-myc alleles, we fused the amino-terminal transactivation domain (amino acids 1-262) of wild type and the four mutant c-myc alleles to the DNA binding domain of the yeast transcription factor GAL4. In a first experiment, we compared expression levels of the various GAL4-myc chimeric proteins. U2-OS osteosarcoma cells were transiently transfected with the wild type and mutant GAL4-myc expression vectors. After two days, cell lysates were prepared from transfected cells and subjected to polyacrylamide gel electrophoresis. The size-fractionated proteins were transferred to a nitrocellulose filter and detected with a polyclonal Myc antibody. As can be seen in Fig. 2, the Myc antibody detects both endogenous c-Myc protein (which provides an internal control for protein loading) and the slightly faster-migrating transfected GAL4-myc fusion protein. Fig. 2also shows that the four mutant GAL4-myc fusion proteins are approximately equally well expressed as GAL4-myc wild type.
Figure 2: Expression of Gal4-Myc fusion proteins. U2-OS osteosarcoma cells were transiently transfected with the various GAL4-myc (GM) chimeric expression vectors. After 2 days, protein lysates were prepared from transfected cells and separated on an SDS-polyacrylamide gel. After this, proteins were transferred to a nitrocellulose filter, and Myc proteins were detected with polyclonal rabbit anti pan Myc antiserum.
Figure 3: Transactivation by GAL4-Myc and repression by p107. A, U2-OS cells were transfected with GAL4 reporter plasmid alone or cotransfected with reporter plasmid and pJ3-GAL4-myc expression vectors with specific missense mutations within the coding region (numbers below bars indicate the position of the mutations in c-Myc; WT, wild type), together with pCMV-p107 sense (gray bars) or p107 antisense (black bars). Data are representative of at least three independent experiments, each performed in duplicate. B, same experiment as in A performed in Chinese hamster ovary cells.
These results are in apparent contrast with earlier studies by Hoang et al.(1995) and Gu et al.(1994) who found that ten different c-Myc alleles from BL cell lines did resist inhibition by p107. Since Hoang et al.(1995) used CHO cells in their studies, we repeated the experiment shown in Fig. 3A in CHO cells. Fig. 3B shows that all four mutant c-Myc chimeric proteins were equally sensitive to p107 suppression in CHO cells as compared to the human osteosarcoma cells. These data indicate that differences in cell type are not likely to be responsible for the observed difference in sensitivity to p107 suppression.
Figure 4: Transactivation by full-length mutant c-Myc proteins. U2-OS cells were transfected with Myc/Max reporter plasmid alone or cotransfected with reporter plasmid and pJ3-myc expression vectors with specific missense mutations within the coding region (numbers below bars indicate the position of the mutations in c-Myc; WT, wild type), together with pCMV-p107 sense (gray bars) or antisense (black bars). Data are representative of at least three independent experiments, each performed in duplicate.
Figure 5: Effect of cyclin-cdks on c-Myc transactivation. U2-OS cells were transfected with GAL4 reporter plasmid alone (column 1) or cotransfected with reporter plasmid and pJ3-GAL4-myc expression vector (column 2), together with pCMV-p107 (columns 3 and 4) and cdk2-dominant negative expression vector (cdk2-DN, column 4). in addition, GAL4-myc was cotransfected with a mutant p107 expression vector that directs the synthesis of a truncated p107 protein unable to bind cyclins (p107-N385, column 5). Data are representative of at least three independent experiments, each performed in duplicate.
Figure 6: p107 phosphorylation is inhibited by dominant negative cdk2. U2-OS cells were transfected with HA-epitope-tagged p107 expression vector (lanes 2-4) in the presence of either cdk4-DN expression vector (lane 3) or cdk2-DN (lane 4). After 2 days, protein lysates were prepared from transfected cells and separated on a SDS-polyacrylamide gel. After this, proteins were transferred to a nitrocellulose filter, and p107 protein was detected with monoclonal antibody 12CA5 directed against the HA epitope of transfected p107.
In a second approach, we used an expression vector that directs the synthesis of an amino-terminally truncated p107 protein. p107-N385 is unable to bind cyclin A-cdk2 complexes (Zhu et al., 1995) and may therefore be unable to inhibit c-Myc transactivation. Fig. 5shows that p107-N385 was more effective than the wild type p107 protein in suppression of c-Myc transactivation. This result further supports the notion that recruitment of cyclin A-cdk2 to c-Myc by p107 is not required to mediate inhibition of transactivation.
We describe here the functional characterization of three mutant c-myc alleles from primary BL in addition to one c-myc mutant derived from a BL cell line. All four mutant BL c-myc alleles were equally active in transactivation and did not differ from wild type c-myc in their sensitivity to suppression of transactivation by p107. These results differ significantly from those of two other studies in which it was shown that ten different mutant c-Myc proteins from BL cell lines were resistant to inhibition of transactivation by p107 (Gu et al., 1994; Hoang et al., 1995). One difference between our study and those of Gu et al. and Hoang et al. is that in our assays we used single missense mutations, three of which were identified in primary BL. In contrast, Hoang et al. (1995) and Gu et al.(1994) used mutant c-myc alleles found in BL cell lines, most of which carried multiple missense mutations scattered throughout the transactivation domain. We focused on c-myc mutations found in primary BL rather than BL cell lines because BL cell lines frequently acquire additional mutations during in vitro cultivation. Thus, BL cell lines derived from the same tumor have been reported to have different mutations (Albert et al., 1994) and the BL cell line CA46 had additional mutations when compared to the primary tumor (Yano et al., 1993). In addition, the translocated c-myc allele in the BL cell line Raji also continues to accumulate mutations in cell culture (Albert et al., 1994). One possible explanation for the difference in results between this study and the two previous studies may be that resistance of c-Myc to p107 suppression is not frequent in primary BL but is a secondary phenomenon that BL tumor cells acquire when they accumulate additional c-myc gene mutations during in vitro cultivation. It remains unclear, however, why the Thr-58 to Ala mutant is resistant to p107 suppression in the study of Hoang et al.(1995), whereas in the same cell type, the same mutant was found to be sensitive to p107 suppression in the present study (Fig. 3B).
The clustering of mutations in exon 2 and especially in the region encoding amino acids 39-63 may suggest that the sequence alterations found are not neutral with respect to c-Myc function but provide a growth advantage to the cells. This region of the c-Myc protein is part of the transcriptional activation domain of c-Myc (Kato et al., 1990). That transactivation by c-Myc is essential, for its transforming activity is supported by several lines of evidence. First, deletions within the amino-terminal transactivation domain severely affect c-Myc transformation (Kato et al., 1990; Stone et al., 1987). Furthermore, Barrett et al.(1992) have demonstrated a correlation between the transcriptional transactivation potency of Myc proteins and their ability to transform. The c-Myc protein is phosphorylated in vivo, and several studies have suggested that c-Myc transactivation and transformation is influenced by phosphorylation (Albert et al., 1994; Gupta et al., 1993; Henriksson et al., 1993; Pulverer et al., 1994; Seth et al., 1991). Importantly, the two major phosphorylation sites in the transactivation domain, Thr-58 and Ser-62, and their flanking amino acids are most frequently affected in BL (Fig. 1). This may indicate that phosphorylation of at least some of these sites leads to down-regulation of c-Myc growth-promoting activity. Consistent with this is the finding that v-myc oncogenes frequently contain mutations in these phosphorylation sites (Frykberg et al., 1987; Symonds et al., 1989). In this study, we found no evidence that BL mutations affect c-Myc transactivation ( Fig. 3and Fig. 4), and similar results have been obtained by two other groups (Gu et al., 1994; Lutterbach and Hann, 1994), whereas two other groups found that mutation of c-Myc phosphorylation sites leads to reduced transactivation ability (Albert et al., 1994; Gupta et al., 1993). Thus, although different constructs and different cell types have been used in different reports, all studies report that the transactivation ability of mutant BL c-Myc proteins is either comparable to that of wild type c-Myc or reduced. The lack of BL mutations with increased transactivation ability raises the possibility that mutation of amino-terminal residues may affect some other aspect of c-Myc physiology other than transactivation. One possibility is that some of the BL-derived mutant c-myc alleles contribute to tumorigenesis because of a reduced ability to induce apoptosis. That Myc-induced apoptosis depends on amino-terminal motifs within c-Myc has recently been demonstrated (Evan et al., 1992). However, all BL mutant c-Myc protein mutants investigated thus far have unaltered ability to induce apoptosis (Hoang et al., 1995). Another possibility is that transrepression by c-Myc is affected by the BL mutations. That transrepression requires the c-Myc amino terminus is supported by several lines of experimentation (Li et al., 1994; Penn et al., 1990a, 1990b; Philipp et al., 1994). It will therefore be worthwhile to study the effects of BL-derived mutant c-Myc proteins in transcriptional repression assays.
The resistance of BL mutant c-Myc proteins to suppression by p107 is not due to a decreased affinity of the mutant c-Myc proteins for p107 (Hoang et al., 1995). It has been suggested that transactivation by wild type c-Myc is down-modulated by an initial phosphorylation of Ser-62 by a cyclin A-cdk2-p107 complex. Subsequently, additional phosphorylation at Thr-58 is allowed by other kinases that inactivate Myc transactivation. BL-derived mutant c-Myc proteins frequently lack phosphorylation of Thr-58, which renders these mutant c-Myc proteins resistant to inactivation by the cyclin A-cdk2-p107 complex (Hoang et al., 1995). Our data do not support this model for two reasons. First, a mutant of p107 that fails to form a stable complex with cyclin A-cdk2 has wild type ability to suppress c-Myc transactivation (Fig. 5). This indicates that cyclin A-cdk2 plays no role in the p107-mediated down-modulation of c-Myc transactivation. Furthermore, a dominant negative mutant of cdk2 that effectively blocks all cdk2 kinase activity in transiently transfected cells ( Fig. 6and van den Heuvel and Harlow(1993)) did not interfere with inhibition of c-Myc transactivation by p107. This further supports the notion that a cyclin A-cdk2 complex does not play a major role in down-modulation of c-Myc transactivation. A prediction of the model proposed by Hoang et al.(1995) would be that Ser-62 and Thr-58 mutants of c-Myc would have an increased transactivation ability by escaping down-regulation by p107. As was discussed above, this is not found (Gu et al., 1994; Lutterbach and Hann, 1994; Albert et al., 1994; Gupta et al., 1993). We favor the view that p107 binds to the c-Myc transactivation domain to prevent it from interaction with proteins that mediate transactivation. We and others have previously shown that c-Myc can interact with the TATA binding protein, and indeed the p107 binding site on c-Myc appears to overlap with that of the TATA binding protein (Hateboer et al., 1993; Beijersbergen et al., 1994; Maheswaran et al., 1994). It should be noted, however, that this fails to explain why BL mutant Myc proteins bind p107 without being sensitive to its inhibitory effect (Gu et al., 1994; Hoang et al., 1995).
The results in the present paper indicate that escape from p107-induced suppression is not a general consequence for all BL-associated c-Myc mutations. It seems more likely that the heterogeneous BL mutations enhance the growth stimulatory ability of the c-Myc protein in different ways, and several mechanisms, operating either singly or in concert, lead to the abnormalities in cell growth found in BL.