Address correspondence to Philippa Marrack, Howard Hughes Medical Institute, Dept. of Immunology, 1400 Jackson St., Denver, CO 80206. Phone: (303) 398-1324; Fax: (303) 398-1396; email: marrackp{at}njc.org
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Abstract |
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Key Words: Bim B cell development IL-7 B cell survival Bcl-2 family
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Introduction |
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IL-7 is produced by stromal cells and epithelial cells in various organs, including the bone marrow (4). It first came to be recognized as a factor that might be important for B cell development in experiments showing that IL-7 could promote the proliferation and differentiation of B cell progenitors in bone marrow cultures (68). Since then, many different types of knockout and transgenic mice have added to our knowledge of the effects of IL-7 on B cell development (912). As a result, it is now thought that IL-7 is required during several stages of B cell development. For example, IL-7 induces some of the steps of B cell differentiation. These include the differentiation of CLPs into pre-proB cells (13) and, by inducing expression of RAGs with consequent construction of a functional µ chain locus, IL-7 promotes the differentiation of proB cells into preB cells (1418). IL-7 also supports the survival of some types of developing B cells and can, in some cases, induce their proliferation (4, 5). Once immature B cells have left the bone marrow they cease to rely on IL-7 for survival or further development. The survival of these more mature B cells is controlled by ligands for the TNF receptorrelated protein, BAFF (also known as Tall-1, BLyS, THANK, and zTNF; reference 19).
Some of these conclusions, however, are controversial. This is for several reasons. First, in some cases, IL-7 can be replaced by other factors. For example, in culture and in very young mice, the effects of IL-7 on developing B cells might be replaced by thymic stromal lymphopoetin (TSLP), a cytokine that binds to a receptor related to that for IL-7 (20, 21). However, no specific role for TSLP has been identified and mice lacking the TSLP receptor have a normal B lymphoid compartment (22). Second, in some cases, IL-7 appears to act in conjunction with other stimuli. For example, the effects of IL-7 on very early lymphocyte precursors also involve fms like tyrosine kinase 3 (Flt3) or IL-11 plus steel factor (2325), and the effects of IL-7 on the pro to preB cell conversion are aided by signaling through the preB cell receptor itself (26, 27). Third, because the development of B cell precursors deprived of IL-7driven signals is substantially blocked at a very early stage, it precludes study of the effects of IL-7 on later stages of B cell development. Finally, it is not always a simple matter to distinguish between the effects of IL-7 on differentiation versus its effects on B cell precursor survival and/or proliferation.
To deal with this last phenomenon, investigators have manipulated factors known to affect lymphocyte survival. These factors include the antiapoptotic Bcl-2 family members Bcl-2, a protein whose expression is increased by IL-7 signaling, and Bcl-xl, as well as their proapoptotic relative, Bim. Overexpression of these two antiapoptotic proteins in B cells has different consequences. Although the number of preB cells increases in mice overexpressing Bcl-xl (28), expression of Bcl-2 has no effects on B cell precursor number, but instead results in increased numbers of mature B cells (29). Mice lacking Bim also contain three- to fourfold more mature B cells than normal animals (30, 31). Because of the potential of IL-7 to increase expression of antiapoptotic Bcl-2 family members and the known interaction between these survival factors and Bim, Bim could play a role in mediating the death of B cells deprived of IL-7. Interestingly, it was recently shown that B cell precursors from mice lacking Bim are resistant to death when cultured in the absence of IL-7 (30). However, analysis of the role of Bim in mediating the death of B cells deprived of IL-7 in vivo has not been published.
To determine the relative effects of IL-7 on B cell precursor survival versus B cell precursor differentiation, we chose to study the requirements for IL-7 in cells that do or do not express Bim. Absence of Bim allows the survival of some B cell precursors in the absence of IL-7 in vitro. However, our results show that lack of Bim does not promote the conversion of lymphocyte precursors to proB cells or the induction of IgM expression by preB cells. Under conditions of limiting IL-7, B cell differentiation continues, with B cells less likely to survive if they express Bim, but not if they lack Bim. Thus, the number of immature B cells in animals is governed to a large extent by IL-7 and its ability to counteract the death-inducing effects of Bim.
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Materials and Methods |
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Cell Sorting and Flow Cytometry Analysis.
For surface staining, cell suspensions were incubated for 15 min on ice with antimouse FcR-2, 2.4G2 to prevent nonspecific binding of antibodies to the Fc receptors on cells. Cells were then washed and incubated on ice with mixtures of labeled antibodies as noted. Antimouse antibodies (BD Biosciences) used for these experiments included antiCD2-PE, antiCD21/CD35-FITC, antiCD23-PE, antiCD24-biotin, antiCD5-PE, antiB220-APC or CyChrome, and antiIgM-FITC or antiIgM-APC. The monoclonal hamster antimouse Bim antibody, Ham 151-149, was made from a hamster immunized with a complex of mouse Bim and Bcl-XL produced in insect cells. The antibody reacts in Western blots and by immunofluorescence with permeabilized B and T cells from Bim+/+, but not Bim/, mice. Cells were permeabilized with 0.03% saponin, incubated with 12.5 µg/ml Ham 151-149, washed thoroughly, and then stained with PE- or APC-coupled antihamster antibodies. After incubation with antibodies, cells were sorted using a MoFlo machine (DakoCytomation) or analyzed on a FACSCalibur machine. Subsequent analyses used CELLQuest software (BD Biosciences) and FloJo (TreeStar).
Carboxyfluorescein Diacetate Succinimidyl Ester (CFSE) Labeling.
Cells were labeled with CFSE (Molecular Probes) as described previously (33). In brief, a stock solution of 5 mM CFSE in DMSO was diluted at 1:10 in serum-free Spinner modified Eagle's medium (SMEM; Biosource International) that was prewarmed to 37°C. B cells were diluted to 5 x 107 cells/ml and incubated with 5 µM CFSE at 37°C for 10 min. Labeled cells were washed twice with SMEM and placed in culture as described above.
Bone Marrow Culture.
Bone marrow cells were isolated and cultured as described previously (34). In brief, bone marrow was obtained from the femurs of 612-wk-old mice. A single cell suspension was prepared, depleted of erythrocytes using buffered ammonium chloride, washed twice in SMEM, and cultured at 5 x 105 cells/ml with 5 ml/well in a six-well Petri dish (7% CO2, 37°C) in SMEM containing 100 U/ml penicillin, 100 µg/ml streptomycin, 50 µg/ml gentamicin, 2 mM L-glutamine, 1 mM sodium pyruvate, 50 µM 2-ME, 10% FBS (Oatlanta Biologicals), and 50100 U of IL-7 derived from culture supernatant of J558L cells transfected with murine IL-7 cDNA (provided by A. Rolink, University of Basel, Basel, Switzerland). Cells were cultured for time points as noted in Fig. 2, washed twice with SMEM, and used in subsequent experiments. Cell viability was assessed using forward scatter and side scatter analysis on the FACSCalibur cytofluorograph.
RNA Purification and Real-Time PCR Analyses.
RNA was purified from bone marrow cells using Trizol (Life Technologies) according to the manufacturer's instructions. cDNAs were synthesized using M-MLV reverse transcriptase according to the manufacturer's instructions (Life Technologies). cDNAs for IL-7 and actin were analyzed by real-time PCR using the TaqMan PCR kit and an ABI 7700 sequence detector thermal cycler according to the manufacturer's instructions (Applied Biosystems), and quantified with Sequence Detection Systems software 1.6.3 (Applied Biosystems). cDNAs were quantified using a real-time PCR probe and primers previously described for IL-7 (35) and actin (36). Analysis of negative control cDNA synthesis in reactions lacking the M-MLV reverse transcriptase did not produce signal within 40 cycles. Additionally, cDNA made from bone marrow of IL-7/ animals failed to produce a signal within 40 cycles, demonstrating that the IL-7 primers and probe are specific for IL-7 cDNA. RNA levels quantified by these methods were normalized to the levels of actin detected for each sample. All samples were performed in triplicate.
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Results |
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The Death of Early B Cells Induced by Lack of IL-7 Is Caused by Bim.
It has been reported previously that lack of Bim promotes survival of preB cells in the absence of IL-7 in vitro (30). To confirm this result and examine the effects of Bim in survival of developing B cells deprived of IL-7, we isolated B220+ IgM pro and preB cells and immature B cell precursors from Bim+/+ and Bim/ mice and cultured them in the absence or presence of IL-7. Cultures were then harvested and B cell survival was monitored (Fig. 2 A).
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Although a straightforward interpretation of the results in Fig. 2 A suggests that IL-7 operates to counteract the death-promoting effects of Bim in pro and/or preB cells, this interpretation is complicated by the fact that IL-7 can promote development of these subsets of B cells. To begin to dissect these events and determine whether lack of Bim could affect the requirement for IL-7 in pro and preB cell development, we isolated B220+ IgM B cells from Bim+/+ and Bim/ mice, labeled the cells with CFSE, and cultured them in the absence or presence of IL-7. After 3 d, we analyzed the cells for proliferation, as assessed by loss of CFSE, and for differentiation into cells expressing IgM, an event that is known to involve IL-7 (13, 14). As shown in Fig. 2 B, the sorted cells did not divide or differentiate unless IL-7 was present. Additionally, the requirements for IL-7 for differentiation and proliferation were unaffected by expression of Bim. Overall, these results show that IL-7 and Bim counteract each other's effects on the survival of pro and preB cells. However, survival alone (promoted by the absence of Bim) is not enough to permit differentiation to IgM expression and proliferation. As reported previously (1214), IL-7 is needed to induce these latter phenomena.
Absence of Bim Does Not Substitute for IL-7 in the Conversion of CLPs to ProB Cells.
IL-7 is needed to promote differentiation at very early stages of B cell development, in the conversion of CLPs to proB cells and at the conversion of pro to immature B cells (1214, 16). To find out whether lack of Bim can substitute for IL-7 in these events, we compared the number of B cells at various developmental stages in the bone marrow of mice expressing or lacking IL-7 and in mice expressing or lacking Bim. Bone marrow cells were isolated from 6-wk-old mice and stained with antibodies against B220, IgM, CD19, and CD2. Immature and mature B cells, identified as cells bearing IgM and intermediate and high levels of B220, respectively (1), could readily be identified in IL-7+/+ Bim+/+ mice (Fig. 3 A, populations 2 and 3). These cells were found at very low percentages in mice lacking IL-7 whether or not the cells also expressed Bim. Likewise, cells expressing B220 but not IgM, most of which are pro and preB cells (1), were present in IL-7+/+ animals and strikingly deficient in mice lacking IL-7 (Fig. 3 A, population 1). Again, absence of Bim had no effect on this deficit.
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These results were perhaps not surprising because lack of IL-7 has recently been reported to interrupt B cell development at the time of conversion of B220 CLPs to B220+ pre-proB cells. Obviously, a block at this stage would inhibit all downstream events. Therefore, we were particularly interested in the effects of Bim deficiency on the very earliest B cell precursor cells, the B220+ IgM CD19 CD2 cells in bone marrow (Fig. 3 B, population 4). The number of these cells was unaffected by the presence or absence of IL-7 or Bim (Fig. 3, B and C). These cells include nonB lineage cells in addition to pre-proB cells (1). So it is difficult to interpret the absence of an effect of IL-7 deficiency in these cells. It appears clear, however, that in the absence of IL-7, there is a block in lymphocyte development during the conversion of CLPs to proB cells that it is not influenced by the loss of proapoptotic Bim.
A final population of cells, bearing B220 and CD2 but lacking IgM and CD19, is also evident in Fig. 3 B (population 7). These cells express neither the granulocyte marker, GR1, nor the ß chain of the T cell receptor (not depicted), and their numbers are unaffected by the absence of IL-7 or Bim. Taken together with the data presented earlier in this paper, these results suggest that IL-7 promotes early B cell differentiation in at least two stages: during the conversion of CLPs to proB cells and at the conversion of proB cells to pre and immature B cells. Lack of Bim does not substitute for IL-7 in either process.
Lack of Bim Increases the Rate at Which Mature B Cells Accumulate in IL-7/ Mice.
Mature splenic B cells appear in very low numbers in mice lacking IL-7 or lacking the ability to signal via the IL-7 receptor (912), whereas B-1type B cells are unaffected by IL-7 deficiency. To determine whether the absence of Bim would modify the number of cells that could accumulate at the mature B cell stage in the absence of IL-7, we analyzed B cells in the spleens and peritoneal lavage fluid of mice lacking IL-7 with or without Bim, and in the spleens of wild-type animals.
In normal animals, mature, follicular B cells increased somewhat in number as mice aged from 4 to 6 wk and remained constant between 6- and 12-wk-old wild-type mice (Fig. 4). As previously reported (9), the spleens of IL-7deficient animals contained very few mature B cells. Their numbers increased slightly as the mice aged. In IL-7deficient mice, the number of mature B cells was increased if the cells also lacked Bim. The differential between IL-7/ B cells expressing or lacking Bim became more evident with increasing age. Peritoneal B-1a cells were unaffected by loss of either IL-7 or Bim (Fig. 4).
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These results indicate that even though there is no demonstrable effect of the absence of Bim on the number of B cells at any stage of development in IL-7/ mice, lack of Bim can to some extent compensate for lack of IL-7, as far as the number of mature B cells are concerned. This could be due to a very subtle effect of Bim on the number of B cell precursors that can develop independently of IL-7. Alternatively, lack of Bim could prolong the life span of B cells that have managed to develop in the absence of IL-7.
Bim/ Cells Survive and Develop Better Than Bim+/+ Cells When IL-7 Is Limiting.
Experiments have shown that availability of IL-7 in normal animals limits the number of B cells that are produced. For example, administration of IL-7, or overexpression of the gene for IL-7, increases the number of B cells in mice (42, 43). In old mice, IL-7 levels in the bone marrow decrease and B cell production is diminished (4445). The experiments described above and elsewhere show that IL-7 is needed both for survival of early B cells and, at several stages, for their differentiation. Our in vitro experiments also show that IL-7 governs survival of early B cells and that at the stages where this applies, survival in the absence of IL-7 can be achieved by lack of Bim. These results lead us to ask whether differentiation or survival of B cells is more affected by low levels of IL-7.
To answer this question we bred mice expressing or lacking Bim and heterozygous for the IL-7 deficiency. To determine whether IL-7 is more limiting in IL-7+/ mice than in wild-type animals, we performed real-time PCR analysis on bone marrow from IL-7+/+, IL-7+/, and IL-7/ mice. We measured IL-7 message and normalized its levels to those of actin. Fig. 5 A shows that the level of IL-7 mRNA in IL-7+/ bone marrow is 60% of that detected in IL-7+/+ marrow. Therefore, gene dosage does have an effect on IL-7 mRNA levels and probably (although this is very difficult to measure in vivo) on IL-7 protein levels.
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Not surprisingly, survival and differentiation in the bone marrow was followed by transport to and accumulation in the spleen. Thus, the spleens of young IL-7+/ Bim/ animals contained normal numbers of mature B cells, whereas these cells were at half normal numbers in the spleens of IL-7+/ Bim+/+ mice (not depicted). Because lack of Bim overcame the partial deficiency of IL-7 in IL-7+/ animals, and Bim affects only the survival of B cells, these results suggested that for early B cells, survival is more dependent on IL-7 levels than on differentiation.
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Discussion |
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Here, we show that Bim probably does not affect any of the differentiation events induced by IL-7 signaling. B cell development is blocked at a very early stage in mice lacking IL-7 and the blockage is not circumvented by the absence of Bim, even though in wild-type mice, cells at these very early stages express Bim, albeit at very low levels. Thus, either IL-7 does not induce survival signals at this stage, survival alone is not sufficient to drive conversion of CLPs to proB cells, or Bim is not the apoptotic protein crucial for death at this stage.
Likewise, IL-7 induces the differentiation of pro and preB cells to the immature B cell stage and consequent IgM expression (1416). Again, lack of Bim was not sufficient to induce this differentiation event, nor would it allow proliferation of B cell precursors, although lack of Bim did allow survival of the preB cells in the absence of IL-7. Thus, simply staying alive is not enough to allow differentiation of the cells. Additional signals are required, and these signals are delivered via the IL-7 receptor.
It is interesting to compare the effects on survival and lack of effects on differentiation and proliferation of Bim and the various antiapoptotic proteins expressed in early B cells. B cell development is fairly normal in at least young mice lacking Bcl-2 (46). Conditional knockout, at the point at which early B cells start to express CD19 (proB cells), of the gene coding for the antiapoptotic protein Mcl-1 causes the death of B cells at that stage (47). This is one of the stages at which lack of Bim compensates for lack of IL-7. Hence, it is likely that in proB cells, IL-7 allows survival by inducing Mcl-1 (47) and the Mcl-1 counteracts the death-inducing effects of Bim. In the absence of Bim, IL-7 and its downstream effector Mcl-1 are not required for survival. Overall, the results here suggest that Bim and IL-7 balance each other's effects on B cell progenitor survival. However, survival alone is not sufficient to allow B cell precursor differentiation from CLPs to proB cells, or from pro to immature B cells. IL-7 itself is needed for these events.
The data presented here do allow us to draw some conclusions about the relative need for IL-7 signaling for differentiation versus survival. The number of B cells at most maturational stages are about half those in wild-type animals in mice that are heterozygous for IL-7 expression. This suggests that levels of IL-7 are accurately reflected in the number of B cells and their precursors. This effect could be due to control by IL-7 on rates of differentiation, on rates of proliferation, or on survival of B cell precursors. The results presented here suggest that levels of IL-7 affect most predominantly the survival of B cell precursors. This interpretation is suggested by the fact that absence of Bim allows normal numbers of B cell precursors and B cells to appear in mice in which IL-7 is limiting, and Bim is known to affect cell survival, not cell proliferation or, as shown here, cell differentiation.
Why would B cell survival be more sensitive to low levels of IL-7 than B cell differentiation or proliferation? This could be explained in several ways. First, in developing B cells, a brief "hit" by IL-7 might be sufficient to drive differentiation or proliferation signals, whereas survival may require IL-7 to be continuously present. Thus, when IL-7 is limiting, the cells might be intermittently deprived of this life-giving cytokine and thus more likely to die. Alternatively, the observations reported here may suggest that low levels of continuous signaling via the IL-7 receptor are sufficient to induce differentiation and proliferation, but not survival. Others have shown that IL-7 acts with other factors at some stages of B cell development. For example, in normal mice, IL-7 and Flt3 ligand act together to stimulate CLP differentiation to proB cells (23). Later in B cell development, the preB cell receptor and IL-7 act synergistically to promote further differentiation of preB cells, and signaling through the preB cell receptor increases the ability of the cell to detect signaling via the IL-7 receptor (27). Therefore, perhaps the greater sensitivity of precursor B cell survival versus differentiation to IL-7 reflects the (untested) idea that survival is stimulated solely by IL-7, whereas other factors act together with IL-7 to promote differentiation.
IL-7deficient mice are profoundly lacking in mature B cells. Lack of Bim counteracts this deficiency to some extent. This could be due to subtle effects of lack of Bim on cell precursors. For example, in the absence of IL-7, Bim/ pro and preB cells might convert to immature B cells at a slightly higher rate than Bim+/+ pro and preB cells, thus slowly giving rise to a larger number of mature B cells as mice age. If this conclusion is correct, it would suggest that survival time is related to the probability that a B cell precursor will convert to the next stage in its development, in the absence of any other signal. However, it is more likely that mature B cells accumulate in the absence of IL-7 if they also lack Bim because Bim is involved in the survival of mature B cells themselves. Isolated mature B cells from normal mice die fairly rapidly in the absence of BlySS/BAFF in culture, whereas mature B cells lacking Bim have a long survival time when cultured in the same manner (unpublished data). It is likely that this could reflect a longer survival time for mature B cells in animals. Hence, in IL-7deficient mice, mature B cells probably accumulate more rapidly if they also lack Bim because lack of Bim promotes the survival of the mature B cells themselves.
Overall, however, the results presented here show that Bim is expressed at most stages of B cell development and that Bim and IL-7 counteract each other's actions in promoting the death versus the survival of B cell precursors at several stages of development. Bim acts solely to affect B cell survival, however, and does not directly affect B cell proliferation or differentiation. Hence, the balance between Bim and IL-7 is crucial to the control of B cell precursor survival and thus total B cell number.
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Acknowledgments |
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This work was supported by United States Public Health Service grants AI-17134, AI-18785, and AI-22295. M. Wang is a National Institute of Child Health and Human Development (NICHD) Fellow of the Pediatric Scientist Development Program (NICHD grant award no. K12-HD00850-17).
The authors have no conflicting financial interests.
Submitted: 7 June 2004
Accepted: 27 September 2004
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References |
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