Correspondence to: Scott C. Kogan, 505 Parnassus Ave., Rm. M-524, University of California at San Francisco, San Francisco, CA 94143-0100. Tel:415-353-1750 Fax:415-353-1106 E-mail:skogan{at}cc.ucsf.edu.
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Abstract |
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The promyelocytic leukemia retinoic acid receptor (PMLRAR
) chimeric protein is associated with acute promyelocytic leukemia (APL). PMLRAR
transgenic mice develop leukemia only after several months, suggesting that PMLRAR
does not by itself confer a fully malignant phenotype. Suppression of apoptosis can have a central role in tumorigenesis; therefore, we assessed whether BCL-2 influenced the ability of PMLRAR
to initiate leukemia. Evaluation of preleukemic animals showed that whereas PMLRAR
alone modestly altered neutrophil maturation, the combination of PMLRAR
and BCL-2 caused a marked accumulation of immature myeloid cells in bone marrow. Leukemias developed more rapidly in mice coexpressing PMLRAR
and BCL-2 than in mice expressing PMLRAR
alone, and all mice expressing both transgenes succumbed to leukemia by 7 mo. Although both preleukemic, doubly transgenic mice and leukemic animals had abundant promyelocytes in the bone marrow, only leukemic mice exhibited thrombocytopenia and dissemination of immature cells. Recurrent gain of chromosomes 7, 8, 10, and 15 and recurrent loss of chromosome 2 were identified in the leukemias. These chromosomal changes may be responsible for the suppression of normal hematopoiesis and dissemination characteristic of the acute leukemias. Our results indicate that genetic changes that inhibit apoptosis can cooperate with PMLRAR
to initiate APL.
Key Words: leukemia, myeloid/leukemia, promyelocytic, acute/leukopoiesis/PML protein/receptors, retinoic acid
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Introduction |
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Many genetic alterations have been associated with acute myeloid leukemia (AML)1 (1) (2). Nevertheless, our understanding of the combinations of changes sufficient to fully transform myeloid cells remains limited. The t(15;17)(q22;q11.2) chromosomal translocation is closely associated with human acute promyelocytic leukemia (APL; reference 3). This translocation fuses the gene encoding promyelocytic leukemia (PML), a protein that limits proliferation and induces apoptosis, with the gene encoding the retinoic acid receptor (RAR
), a hormone receptor that represses transcription in the absence of retinoic acid and activates transcription in response to this ligand. A PMLRAR
fusion protein is expressed in almost all cases of APL, and this protein can initiate acute leukemias with promyelocytic features when expressed in mice (4) (5) (6).
PMLRAR is thought to contribute to leukemogenesis primarily by inhibiting neutrophilic differentiation. Retinoids can induce differentiation of myeloid and other cell types (7). PMLRAR
inhibits differentiation of myeloid cell lines (8) (9) (10) (11), and all-trans retinoic acid (tRA) binding to PMLRAR
results in transcriptional activation and neutrophilic differentiation (3) (12) (13) (14). Nevertheless, mice expressing PMLRAR
exhibited only mild abnormalities before the appearance of acute leukemia (which arises with limited penetrance only after several months; references 46), suggesting that additional genetic changes cooperate with PMLRAR
to block differentiation.
PMLRAR may also contribute to leukemogenesis by enhancing the survival of immature myeloid cells. Whereas PMLRAR
induces apoptosis of nonhematopoietic and some hematopoietic cell lines (15), PMLRAR
confers increased resistance to apoptosis in myeloid cell lines in which its expression is tolerated (8) (16). PMLRAR
also enhances survival of primary myeloid CFU in response to proapoptotic stimuli (17) and hematopoietic progenitor cells after growth factor deprivation (18). PMLRAR
-mediated suppression of apoptosis might influence the ability of this fusion protein to initiate leukemia.
BCL-2 protects cells from apoptosis by inhibiting the activation of caspases necessary to execute a cell death program (19). In follicular lymphoma, BCL-2 is overexpressed as a result of a t(11;14)(q32;q21) chromosomal translocation. BCL-2 expression has also been observed in AMLs, including leukemic cells of some APL patients, and such expression has been associated with poor prognosis (20) (21) (22) (23) (24) (25) (26). Thus, BCL-2, or related proteins, may play a role in the pathogenesis of a subset of APL and might influence the response of patients to therapy.
Transgenic mice expressing PMLRAR under the control of the MRP8 promoter were bred with MRP8-BCL-2 transgenic mice to assess whether BCL-2 could cooperate with PMLRAR
to initiate leukemia. We observed that coexpression of BCL-2 and PMLRAR
caused a marked accumulation of immature myeloid cells. Furthermore, BCL-2 accelerated the development of acute leukemia in mice that express PMLRAR
.
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Materials and Methods |
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Mice.
Mice were bred and maintained at the University of California at San Francisco and their care was in accordance with University of California at San Francisco guidelines. MRP8-PMLRAR transgenic mice (4) were bred with MRP8-BCL-2 transgenic mice (27) to generate the litters of control, singly transgenic, and doubly transgenic mice used for experiments.
Preparation of Tissues for Analysis.
Blood was obtained from anesthetized animals by venipuncture of the retroorbital venous plexus. Bone marrow was obtained by flushing HBSS through mouse long bones. Blood smears and bone marrow smears were prepared according to standard hematological techniques. Sternums were decalcified for 23 h (formic acid 11%, formaldehyde 8%). Sternums, livers, spleens, and kidneys were fixed overnight in buffered formalin and embedded in paraffin before sectioning.
Peripheral Blood Counts and Bone Marrow Differential Counts. Blood counts of nonleukemic, preleukemic, and some leukemic mice were obtained on automated hematology analyzers running veterinary software (Cell-Dyne3500, Abbott; Hemavet 850, CDC Technologies). Blood counts of leukemias that arose early in the study were obtained on a Technicon H-3 automated hematology analyzer running the standard software used for clinical analysis. Peripheral blood differential white blood cell counts (total of 200 cells each) and bone marrow differential counts (total of 400 cells each) were performed on stained smears as described (28).
Analysis of Proliferation.
Bone marrow cells were fixed in ice-cold 70% ethanol for 30 min. After two washes in PBS, cells were resuspended in PBS containing 50 µg/ml propidium iodide (Boehringer) and 10 µg/ml RNase (Sigma-Aldrich). After a 30-min incubation, cells were analyzed using a FACScanTM flow cytometer (Becton Dickinson) and cell cycle distribution of 10,000 events was assessed using Modfit software (Becton Dickinson).
Analysis of Apoptosis.
Immediately after harvest, bone marrow cells were washed twice in PBS with 2% heat-inactivated fetal bovine serum (wash buffer), and cells were then stained with FITC-conjugated antibodies to CD18 or an isotype control (BD PharMingen) for 20 min on ice. Then, cells were washed and stained for 30 min in the dark, on ice, with 20 µg/ml 7-amino actinomycin D (7-AAD; Calbiochem). After being washed twice, cells were resuspended in wash buffer containing 10 µg/ml actinomycin D (Calbiochem). Analysis was carried out using a FACScanTM flow cytometer within 1 h of staining. 50,000 events were analyzed using CELLQuestTM software (Becton Dickinson). CD18+ cells were gated and three populations were identified: 7-AADlow live nonapoptotic cells; 7-AADmoderate apoptotic cells; and 7-AADbright dead cells (29).
Methylcellulose Cultures of Bone Marrow.
As described previously (28), bone marrow cells were cultured in duplicate in 35-mm petri dishes in Methocult M3230 methylcellulose medium (StemCell Technologies Inc.) supplemented with either 50 U/ml of G-CSF (Boehringer) or 20 ng/ml GM-CSF (StemCell Technologies Inc.). 1-ml cultures contained 50,000 viable bone marrow cells. Cultures were examined at 7 d. Colonies were counted on an inverted light microscope. Duplicate plates were averaged. Cells were harvested, pelleted, washed once in HBSS, and counted before preparation of cytospins. Differential cell counts (total of 200 cells each) were performed on stained cytospins to assess percentages and calculate absolute numbers of neutrophilic cells. To assess the effects of growth factor deprivation, cells were placed into methylcellulose medium with or without GM-CSF and incubated for 24 h before plating matched cultures in the presence of GM-CSF. Results were expressed as a percentage (CFU of growth factordeprived culture/CFU of matched culture without growth factor deprivation x 100).
Transplantation of Bone Marrow.
Essentially as described previously (4), total bone marrow isolated from tibias and femurs of 46-wk-old mice was divided for intravenous injection into 610 recipient mice (13 x 106 nucleated marrow cells/recipient). 612-wk-old FVB/N mice were prepared for transplantation by cesium irradiation totaling 10 Gy, divided into two doses 36 h apart. The results shown in Fig 3 include five recipients of PMLRAR
/BCL-2 doubly transgenic marrow that was 0.75 FVB/N strain, 0.25 BA strain; six recipients of matched PMLRAR
singly transgenic marrow (0.75 FVB/N, 0.25 BA); eight recipients of PMLRAR
/BCL-2 doubly transgenic marrow (0.98 FVB/N, 0.02 BA); and 21 recipients of PMLRAR
singly transgenic marrow (1.0 FVB/N). The difference in survival of recipients of doubly transgenic and singly transgenic marrow was statistically significant whether the data were analyzed as a whole or as subgroups.
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Comparative Genomic Hybridization.
Comparative genomic hybridization was performed as described previously (30) (31) at the Molecular Cytogenetics Core Facility, Comprehensive Cancer Center, University of California at San Francisco.
Retinoic Acid/Arsenic Treatment.
As described previously, mice were treated by subcutaneous implantation of a 21-d release pellet containing 5 mg tRA or placebo (Innovative Research of America; reference 4), and/or by daily intraperitoneal injection of As2O3 (arsenic) at a dose of 5 µg/g body wt (32).
Statistical Analysis.
The software program Statistica (v.4.1 for Macintosh) was used to prepare Kaplan-Meier curves and to compare survival using the Wilcoxon test. Other statistical analyses were performed with Excel (v.5.0/95) using the Student's t test, two-tailed distribution, and unequal variance. Comparisons are with control animals unless otherwise noted.
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Results |
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BCL-2 Cooperates with PMLRAR to Impair Neutrophil Maturation and Expand Myeloid Progenitors.
Previously, we developed a mouse model of APL by expressing PMLRAR in the neutrophilic cells of transgenic mice (4). PMLRAR
had a modest effect on neutrophil differentiation but did not initially arrest maturation. Some of the PMLRAR
transgenic mice went on to develop acute leukemia with promyelocytic features. The latency and limited penetrance of the leukemic phenotype indicated that in this mouse model, additional events were required to cooperate with PMLRAR
in the genesis of acute leukemia. In our effort to identify genetic changes that can cooperate with PMLRAR
to induce leukemia, we considered previous studies indicating that PMLRAR
induces apoptosis of many cell lines (15) and evidence that apoptosis can be a critical regulator of malignant transformation in vivo (33).
To assess the hypothesis that suppression of apoptosis cooperates with PMLRAR in leukemogenesis, we crossed MRP8-PMLRAR
transgenic mice with MRP8-BCL-2 transgenic mice (27). Previous studies of MRP8-BCL-2 transgenic mice indicated that (a) the BCL-2 transgene inhibited apoptosis of neutrophils but not their engulfment by macrophages (27), (b) the transgene inhibited apoptosis of monocytes as well as rescued macrophages and partially reversed osteopetrosis in op/op mice (34), (c) the transgene inhibited Fas-induced apoptosis of myeloid progenitors (35), and (d) in the context of FASlpr/lpr mice, the BCL-2 transgene contributed to the development of a lethal proliferation of myeloid cells (35). These results showed that the BCL-2 transgene was able to suppress apoptosis of myeloid cells and contribute to myeloid neoplasms.
MRP8-BCL-2 transgenic mice were mated with MRP8-PMLRAR mice to examine the effects of the combination of transgenes on hematopoiesis. In the peripheral blood, total leukocyte counts and hemoglobin levels of 35-wk-old transgenic mice were normal (Fig 1 A). Singly transgenic mice had normal platelet counts, whereas those of doubly transgenic mice were elevated. PMLRAR
transgenic mice had normal peripheral blood neutrophil counts, but mice expressing BCL-2 alone or in combination with PMLRAR
were neutropenic (Fig 1 B). Decreased neutrophil counts were previously observed in MRP8-BCL-2 transgenic mice (34). In the bone marrow, both PMLRAR
and BCL-2 singly transgenic mice exhibited a shift from mature neutrophilic cells to immature neutrophilic cells with a small increase in promyelocytes. Doubly transgenic mice had very few neutrophilic cells beyond the promyelocyte stage (Fig 1 C). Whereas the bone marrow of singly transgenic mice looked modestly different from control mice (Fig 2AC), doubly transgenic bone marrow was filled with immature cells and morphologically resembled acute leukemia (Fig 2 D). However, unlike leukemic animals, the organs of these doubly transgenic mice had a near normal appearance (Fig 2EJ).
We also assessed proliferation and apoptosis in the transgenic mice (Table 1). PMLRAR did not discernibly alter the number of proliferating or apoptotic cells detected in bone marrow. BCL-2 increased the number of proliferating cells, and the combination of transgenes increased both proliferation and apoptotic cell numbers. Bone marrow histology provided additional evidence of increased cell turnover in doubly transgenic bone marrow; compared with control, increased numbers of tingible body macrophages were present (Fig 2K and Fig L). The increased proliferation in doubly transgenic mice is consonant with the presence of increased promyelocytes because promyelocytes, unlike mature neutrophils, are mitotically active. The increase in apoptotic cells likely reflects the fact that in some settings, such as growth factor deprivation, BCL-2 delays but does not prevent cell death (36). The combination of BCL-2 and PMLRAR
caused an accumulation of numerous immature myeloid cells in the bone marrow. These cells could proliferate, but very few differentiated into mature neutrophils. BCL-2 appeared unable to block indefinitely the death of the resulting expanded promyelocyte population.
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Methylcellulose cultures were performed to examine the effects of the transgenes on myeloid colony formation in vitro (Table 2). PMLRAR did not alter the number of colonies formed in GM-CSF or G-CSF. In contrast, BCL-2 resulted in increased colonies, an effect that was statistically significant for doubly transgenic bone marrow. The effect of growth factor deprivation on CFU was also assessed for singly transgenic mice. Matched GM-CSF cultures of control, PMLRAR
, and BCL-2 bone marrow cells were plated with or without 24 h of growth factor deprivation. Both PMLRAR
and BCL-2 resulted in a trend towards enhanced survival (control 61 ± 7%, n = 6; PMLRAR
77 ± 17%, n = 6, P = 0.07; BCL-2 95 ± 14%, n = 4, P = 0.01). With regard to differentiation, PMLRAR
, BCL-2, and PMLRAR
/BCL-2 transgenic bone marrows gave rise to a decreased percentage of neutrophils, accompanied by increased immature and monocytic cells. Of note, although the combination of BCL-2 and PMLRAR
caused profound neutropenia in vivo, neutrophil maturation was not completely blocked in bone marrow cultures. In GM-CSF, absolute numbers of neutrophils in BCL-2 and PMLRAR
/BCL-2 cultures were normal because increased colony numbers offset the relative decrease in neutrophil maturation. However, in G-CSF absolute numbers of neutrophils were decreased. These results suggest that PMLRAR
and BCL-2 impeded neutrophil differentiation of myeloid precursors. Altogether, our observations of doubly transgenic animals showed that BCL-2 expanded myeloid progenitors, allowed increased numbers of cells to proliferate, and enhanced the ability of PMLRAR
to inhibit neutrophil differentiation.
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BCL-2 Cooperates with PMLRAR to Initiate Leukemia.
The experiments described above were performed on matched 35-wk-old littermates. We noted that mice that inherited both transgenes were smaller than littermates at 3 wk of age, had the skin abnormalities we have seen in our PMLRAR transgenics (4), and died between 4 and 6 wk of age. To assess the degree to which these deaths were due solely to a hematopoietic disorder or in part to nonhematopoietic effects of the transgenes, we harvested bone marrow from doubly transgenic mice and used this marrow to reconstitute lethally irradiated nontransgenic animals. Marrow harvested from PMLRAR
singly transgenic mice was similarly transplanted. Transplantation of either PMLRAR
transgenic or PMLRAR
/BCL-2 doubly transgenic bone marrow rescued recipient mice from lethal irradiation. Recipients remained healthy for 3 mo or more after transplantation, suggesting that the early deaths of untransplanted doubly transgenic mice were, at least in part, caused by nonhematopoietic effects of the transgenes.
Mice reconstituted with PMLRAR or PMLRAR
/BCL-2 bone marrow were observed for the development of leukemia. Leukemias developed more rapidly in mice coexpressing PMLRAR
and BCL-2 than in mice expressing PMLRAR
alone (median time to leukemia 127 vs. 257 d; Fig 3). All mice reconstituted with doubly transgenic bone marrow succumbed to leukemia by 196 d of age. Similar to the leukemias that arose from singly transgenic PMLRAR
mice, leukemias arising from PMLRAR
/BCL-2 doubly transgenic mice were characterized by anemia and thrombocytopenia, and by bone marrow that was effaced by cells at the blast-promyelocyte stage of differentiation (Fig 4 and Fig 5 A). Although there was a trend towards increased peripheral white blood cell counts in PMLRAR
/BCL-2 leukemias, this trend was not statistically significant (P > 0.05).
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Dissemination Appears to Be a Central Characteristic of AML.
PMLRAR/BCL-2 transgenic mice had bone marrow that morphologically resembled acute leukemia (Fig 2 D and 5 A), yet mice whose bone marrow expressed both transgenes did not become ill for a period of 37 mo. Therefore, we sought to identify differences between preleukemic and overtly leukemic, doubly transgenic animals. Bone marrow differential counts showed very low numbers of maturing neutrophils in preleukemic and leukemic animals (Fig 1 C, PMLRAR
/BCL-2; Fig 4 B). However, in the leukemias suppression of normal hematopoiesis was evident: there was a marked decrease of nucleated erythroid cells in the bone marrow, and in contrast to preleukemic animals, the leukemic mice were anemic and thrombocytopenic (Fig 1 A and 4 A). Furthermore, in the leukemic mice, immature neutrophilic cells were disseminated. Small numbers of promyelocytes were present in the peripheral blood, and the spleens, livers, and kidneys in leukemic mice were enlarged and contained infiltrates of leukemic cells (Fig 5BD). The existence of a prolonged preleukemic state in PMLRAR
/BCL-2 mice suggests that the suppression of normal hematopoiesis and dissemination of leukemic cells observed in AML are not a direct consequence of arrested differentiation.
Acquired Chromosomal Abnormalities Are Common in Murine APL.
Preleukemic, doubly transgenic mice initially produced adequate red blood cells and platelets and did not become ill for 37 mo. These findings indicated that the combination of BCL-2 and PMLRAR was sufficient to initiate but not complete leukemic transformation. Therefore, we sought to identify additional genetic changes in our leukemias. Comparative genomic hybridization was performed on 30 murine APLs, including 20 PMLRAR
leukemias and 10 PMLRAR
/BCL-2 leukemias. Chromosomal copy number abnormalities were observed in 17/20 PMLRAR
leukemias and 9/10 PMLRAR
/BCL-2 leukemias. Gain of chromosomes 7, 8, 10, and 15 and loss of chromosome 2 occurred in three or more samples including both PMLRAR
and PMLRAR
/BCL2 leukemias (Fig 6). Losses of the X chromosome from female samples and the Y chromosome from male samples were also observed. These results identify chromosomal regions whose loss or gain may complete the process of leukemic transformation initiated by PMLRAR
.
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Murine APL Expressing BCL-2 Responds to Retinoic Acid and Arsenic Trioxide.
We assessed whether the expression of BCL-2 influenced the ability of tRA therapy to cause differentiation and prolong survival of mice with APL. Nontransgenic mice received intravenous injections of 5 x 106 spleen cells from leukemia 2995A4, which expresses both PMLRAR and BCL-2 transgenes. In one experiment, 32 d after the injection of leukemic cells, three mice were treated with placebo and three with tRA. The placebo-treated mice died on days 3 and 5, and five died after initiation of therapy, whereas tRA-treated mice died on days 17, 25, and 33. The difference in survival was significant (P = 0.04). In a second experiment, groups of six mice were treated 14 d after the injection of leukemic cells; again, tRA prolonged survival (Fig 7 A). The prolongation in survival we observed (median 42 d, range 1173) was comparable to the increase in survival seen in recipients of a PMLRAR
leukemia that was similarly treated (median 41 d, range 33175; reference 32). tRA induced neutrophilic differentiation of leukemic blasts coexpressing PMLRAR
and BCL-2 (Fig 7 B), but did not abrogate expression of the transgenes as assessed by Western blot analysis (data not shown).
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We also examined whether arsenic and tRA were an effective combination therapy for APL expressing BCL-2. In three experiments, nontransgenic mice received intravenous injections of 107 leukemic 2995A4 cells. After 15 d, mice were treated with tRA and/or arsenic for 4 d, two mice per group, and then killed. Similar to what was previously observed for murine APL that does not express BCL-2 (32), arsenic-induced apoptosis and some differentiation, and the combination of arsenic and tRA, caused rapid regression of the leukemia. 4 d of therapy decreased spleen size (control, 0.57, 0.46 g; tRA, 0.21, 0.20 g; arsenic, 0.40, 0.30 g; tRA/arsenic: 0.10, 0.09 g; representative data from one of three experiments). In the liver, tRA caused regression but not the disappearance of disease, and the addition of arsenic eliminated the visible leukemic cell population (Fig 7 C). These results suggest that APL cells expressing BCL-2 remain sensitive to arsenic plus tRA combination therapy.
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Discussion |
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Expression of BCL-2 in mice that also express the APL-associated PMLRAR fusion protein caused a marked accumulation of immature myeloid cells and accelerated the development of leukemia. Progression from preleukemia to acute leukemia was characterized by suppression of normal hematopoiesis and dissemination of leukemic cells. Additional genetic changes accompanied this transition from abnormal neutrophil maturation to lethal disease.
A Role for Suppression of Apoptosis in APL Pathogenesis.
The possible role of apoptosis in APL pathogenesis has been unclear. Whereas PMLRAR induces cell death in many cell lines, it also inhibits apoptosis of some myeloid cell lines and primary myeloid cells. We anticipated that BCL-2 might cooperate with PMLRAR
to initiate leukemia. On the other hand, given the ability of PMLRAR
itself to block apoptosis, it was possible that BCL-2 would have little impact on leukemogenesis. We observed that the antiapoptotic protein BCL-2 did cooperate with PMLRAR
to initiate leukemia, indicating that genetic changes that suppress apoptosis can cooperate with the PMLRAR
fusion in APL.
The MRP8-BCL-2 transgene has been demonstrated to increase survival of myeloid cells (27, 34, 35, and our results). We observed increased CFU and young myeloid forms in bone marrows of BCL-2 and doubly transgenic mice. It is likely that this increase is in part attributable to the ability of BCL-2 to enhance survival of immature myeloid cells. BCL-2 makes cells less dependent on external survival signals. BCL-2 did not, however, permit unlimited survival of immature cells. We speculate that the preleukemic, doubly transgenic cells remained responsive to extracellular signals that limited their expansion to hematopoietic microenvironments. Nevertheless, it appears that by expanding the population of immature myeloid cells in PMLRAR transgenic mice, BCL-2 made it inevitable that additional leukemogenic mutations would accumulate. Expression of BCL-2 therefore promotes promyelocyte transformation but is not sufficient to complete this process. Interestingly, whereas BCL-2 may facilitate the acquisition of genetic changes that induce acute leukemia in PMLRAR
transgenic mice, it does not appear to alter the type of chromosomal changes that occur.
Cytogenetic Changes in Murine APL.
The t(15;17) translocation is present as an isolated karyotypic abnormality in the majority of APL patients at presentation. However, additional karyotypic abnormalities are observed in 2439% of untreated APL patients (37) (38) (39) (40). The fact that a substantial minority of new APL cases have additional cytogenetic changes provides evidence that human APL results from a combination of acquired mutations. The most common additional abnormality is trisomy 8, which is seen in 17% of patients at presentation. Other recurrent aberrations include loss of chromosome 9q and isochromosome of the long arm of the derivative chromosome 17. The particular genes through which these additional cytogenetic changes may contribute to leukemia have not been identified.
Some of the changes seen in murine APL correspond to karyotypic abnormalities in human APL. Murine chromosomes 8 and 15 contain regions homologous to human chromosome 8. The area of loss we noted on mouse chromosome 2 contains genes that in humans are located on human chromosome 9q. In the broader context of attempts to understand leukemia pathogenesis in mice, the gain of chromosome 15 and the loss of chromosome 2 have been observed previously. Gibbons et al. (41) observed a common gain of chromosome 15 in B/myeloid leukemias that arose in irradiated Eµ-BCL-2 mice. The authors suggested that the presence of BCL-2 permitted cells damaged by radiation to tolerate chromosomal damage, and the subsequently damaged cells gave rise to the observed leukemias. In our experiments, BCL-2 could have similarly tolerized early myeloid cells to spontaneous genetic changes including a pathogenic gain of chromosome 15. Loss of murine chromosome 2 has been observed in radiation-induced myeloid leukemias in mice (for a review, see reference (42)). The region of murine chromosome 2 identified in these leukemias was lost in all four APLs in which we observed copy number changes on chromosome 2. Of interest, another group studying the effects of PMLRAR, under the control of a different promoter in a different strain of mice, has also identified recurrent gain of chromosome 15 and recurrent loss of chromosomes 2, X, and Y in their leukemias (43). The chromosome copy number abnormalities observed in murine APLs may facilitate identification of genetic changes that cooperate with PMLRAR
to cause acute leukemia.
BCL-2 Effects on Neutrophil Differentiation.
Although PMLRAR can inhibit differentiation, its effects on neutrophilic differentiation of primary bone marrow cells were modest and most apparent in vitro (Table 2). In vivo, BCL-2 cooperated with PMLRAR
to block maturation at the promyelocyte stage. Given the central role of BCL-2 family members in regulating cell death, the inhibition of neutrophil differentiation in PMLRAR
transgenic mice brought by coexpression of BCL-2 is likely an indirect effect of BCL-2. Enhanced survival of neutrophil precursors may abrogate signals within the bone marrow that normally stimulate promyelocytes to differentiate into mature neutrophils. The finding that mature erythroid cells stimulate the death of erythroid progenitors (44) raises the possibility that interactions between mature and immature myeloid cells play a role in neutrophil maturation. Such interactions could be disrupted by enhanced survival of immature elements. On the other hand, our data are consistent with the speculative idea that BCL-2 may directly influence neutrophil maturation. Our finding that BCL-2 transgenic marrow gave rise to relatively decreased neutrophils in vitro might reflect enhanced production of monocytic cells, but, alternatively, this decrease could reflect a cell autonomous effect of BCL-2 on neutrophil differentiation. In previous studies, BCL-2 did not block tRA-induced differentiation of HL-60 cells (45), but BCL-2 did delay neutrophilic maturation of 32DCl3 cells in response to G-CSF (46). Another finding suggesting that, in some settings, BCL-2 family members might directly influence neutrophil differentiation is the observation that tRA-mediated differentiation of APL cells is accompanied by caspase activation (13). BCL-2 family members might influence differentiation through an activity that is distinct from their effects on cell survival. Such a possibility has precedent: BCL-2 has an effect on proliferation separable from its effect on survival (47).
Multistep Pathogenesis for APL.
The pathogenesis of human APL may parallel that of murine APL. The acquisition of the t(15;17)(q22,q11.2) with resulting expression of PMLRAR could initiate leukemia. Increased expression of BCL-2, or other genetic changes that enhance survival and impair differentiation of the initiated cells, may occur in some patients and facilitate the acquisition of genetic changes that result in acute leukemia. Further study of human APLs could inform our understanding of the role of BCL-2like proteins in the human disease. Although BCL-2 expression was not seen in one study of APL cases (21), subsequent reports indicated that BCL-2 is expressed in most APLs (22) (23) (24) (25) (48). Elucidating whether this BCL-2 expression is because of a genetic lesion in the BCL-2 gene or a downstream result of other lesions should be of value, as should assessing the expression of other BCL-2 family members in APL.
It is notable that the t(15;17) translocation is likely to have effects that are more pronounced than those caused by PMLRAR alone. Similar to BCL-2 expression, loss of Pml, a genetic event that suppresses apoptosis, facilitated the development of acute leukemia in CathepsinG-PMLRAR
transgenic mice (49). The reciprocal fusion protein, RAR
PML, also increased the penetrance of leukemia in mice expressing PMLRAR
(50). Given the fact that the incidence of t(15;17)-associated myeloid leukemia does not increase with age (51), we favor a model in which the translocation initiates the disease and additional required genetic changes may accumulate in a relatively brief period of time.
BCL-2 Does Not Block the Response to APL Therapy.
Downregulation of BCL-2 accompanies the differentiation of APL cells that is induced by tRA (52), and this downregulation may be important for some effects of tRA (13). We found that overexpression of BCL-2 did not block the differentiative effect of tRA. Similarly, BCL-2 might have blocked the therapeutic effect of arsenic because arsenic is thought to induce remissions primarily by stimulating apoptosis of the APL blasts (53) (54) (55). The fact that murine APL overexpressing BCL-2 still responded to arsenic suggests that arsenic can overcome a BCL-2mediated delay in apoptosis. This result is also consistent with the hypothesis that differentiative effects of arsenic contribute to its therapeutic value. Although we studied the response of a single transplantable PMLRAR/BCL-2 leukemia to tRA and arsenic and, therefore, have not addressed possible heterogeneity among such leukemias, our results nevertheless indicate that BCL-2 expression can be associated with an intact response. Thus, human APLs that overexpress BCL-2 or have acquired analogous changes may remain responsive to the novel APL therapies, tRA and arsenic.
Is Dissemination of Myeloid Leukemia Cells the Equivalent of Metastasis of Solid Tumors?
Discussions of AML pathogenesis often focus on the inhibition of differentiation characteristic of the disease. The existence of a preleukemic state in PMLRAR/BCL-2 transgenic mice characterized by maturation that is nearly arrested suggests that additional features of AML, including suppression of normal hematopoiesis and dissemination of leukemic cells, are not the direct result of inhibited differentiation. AML may result from two fundamental abnormalities: (a) a relative inhibition of differentiation that is accompanied by (b) a relative autonomy that allows the leukemic cells to survive and proliferate outside of their normal microenvironment. The idea that survival and proliferation outside of the normal microenvironment are central to AML parallels the concept that for solid tumors, invasion and metastasis define malignancy. In our APL model, although BCL-2 enhances cell survival, other genetic lesions are still required to fully overcome normal growth controls.
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Footnotes |
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1 Abbreviations used in this paper: 7-AAD, 7-amino actinomycin D; AML, acute myeloid leukemia; APL, acute promyelocytic leukemia; PML, promyelocytic leukemia; RAR, retinoic acid receptor
; tRA, all-trans retinoic acid.
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Acknowledgements |
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The authors thank Anne Janin and Hugues de Thé for their assistance with arsenic studies; Lois Koren-Serxner, Gayatry Mohapatra, and Meijuan Zhou for their assistance with mice and DNA preparation; Bob Flandermeyer, Gregg Magrane, and Fred Waldman of the University of California at San Francisco Comprehensive Cancer Center Molecular Cytogenetics Core Facility for comparative genomic hybridization; Daniel Stites and Frank McCormick for their continuing support; and H. Jeffrey Lawrence and Daphne Haas-Kogan for critical comments on the manuscript.
This work was supported by grants CA4338 and CA75986 from the National Institutes of Health and funds from the G.W. Hooper Research Foundation. S.C. Kogan is a recipient of a Burroughs Wellcome Fund Career Award and is an Edward Mallinckrodt Jr. Foundation Scholar.
Submitted: 21 August 2000
Revised: 22 December 2000
Accepted: 9 January 2001
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References |
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