B cell development and activation defects resulting in xid-like immunodeficiency in BLNK/SLP-65-deficient mice
Shengli Xu,
Joy En-Lin Tan,
Esther Poh-Ying Wong,
Arunkumar Manickam,
Sathivel Ponniah and
Kong-Peng Lam
Institute of Molecular and Cell Biology, National University of Singapore, 30 Medical Drive, Singapore 117609, Republic of Singapore
Correspondence to:
K.-P. Lam
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Abstract
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Engagement of the B cell receptor (BCR) leads to the activation of tyrosine kinases and other signaling molecules that ultimately determine the type and magnitude of the B lymphocyte's cellular response. The adaptor protein BLNK/SLP-65 plays a pivotal role in BCR signal transduction by coupling Syk activation to downstream elements such as Grb2, phospholipase C-
, Vav and Nck. We have generated BLNK/ mice to determine the physiological role of this protein in B cell development and activation. BLNK/ mice exhibit an incomplete block in B cell development with a severe inhibition of pro-B to pre-B cell differentiation. BLNK/ sIgM+ cells can develop, seed the peripheral lymphoid tissues and accumulate in numbers overtime. However, these mutant B cells failed to mature and are non-responsive to BCR cross-linking in terms of proliferation and up-regulation of activation markers such as CD69 and CD86 (B7-2). In addition, the CD5+ subset of B cells is absent. The immune response to T cell-independent antigen but not T cell-dependent antigen is also impaired. Overall, the phenotype of BLNK/ mice bears a striking resemblance to that of xid mice which is the murine model of human XLA that has a mutation in Bruton's tyrosine kinase. This raises the interesting possibility that mutation in BLNK/SLP-65 may be responsible for certain human immunodeficiencies.
Keywords: adaptor protein, B cell antigen receptor, CD5+ B cells, signal transduction, gene targeting
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Introduction
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The pre-B cell receptor (pre-BCR) and the BCR play pivotal roles in the development of B lymphocytes. The pre-BCR comprising the Ig heavy chain and surrogate light chains, and the BCR that is composed of the surface Ig, are complexed to the signal transducing subunits Ig
and Igß (1). Studies with the µMT mouse that has a targeted deletion of the transmembrane exon of the Ig heavy chain (2) or the
5T mouse that lacks surrogate light chain (3) indicated that the inability of these mutant mice to express a pre-BCR can lead to the arrest of B cell development at a very early stage. In addition, mice with a compromised BCR resulting from the truncation of the cytoplasmic tail of Ig
(4) do not accumulate mature B cells in the periphery. Finally, the induced ablation of BCR on mature peripheral B cells leads to their rapid cell death (5). Taken together, these studies implied that signals from the pre-BCR and BCR are required for the progression of B lymphopoiesis and the maintenance of B cell survival.
Signal transduction events have been studied extensively in B lymphocytes. Engagement of the BCR activates cytoplasmic protein tyrosine kinases such as Syk, Lyn, Blk and Bruton's tyrosine kinase (Btk) (6), and can lead to a multitude of cellular responses, such as proliferation, activation, differentiation or cell death. The current challenge in the field of B cell signaling is to identify specific signaling pathways that associate with a particular cellular response. Recently, it has been demonstrated that adaptor proteins play a major role in interfacing tyrosine kinase activation by lymphocyte antigen receptors with selective downstream signaling molecules. One such adaptor molecule termed BLNK (7), SLP-65 (8) or BASH (9) has been identified in B cells and is specifically involved in BCR signaling. BLNK can associate with Btk (10) and also couple Syk activation to Grb2, phospholipase C (PLC)-
, Vav and Nck (7), and is intimately associated with intracellular Ca2+ mobilization which is essential for cell activation (11).
BLNK contains a C-terminus SH2 domain, several SH3 domains and a series of YXXP motifs in the N-terminus (79). It bears striking homology to another adaptor protein SLP-76 that is expressed in T cells (12) and intimately involved in TCR signaling. In general, the order of the signaling events from the TCR and BCR is quite similar, with the engagement of the antigen receptors triggering the activation of similar classes of intracellular cytoplasmic kinases. In analogy to BLNK in B cells, SLP-76-coupled TCR induced ZAP-70 (the equivalent of Syk) activation to Ca2+ mobilization in T cells (13). In addition, SLP-76 is essential for T cell development as its inactivation in the mouse germline leads to a profound block in thymocyte maturation at a very early stage (14,15). Thus, given the central role of BLNK in BCR signaling and its similarity to SLP-76 in T cells, we have inactivated BLNK in the mouse to study its physiological role in B cell development and activation.
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Methods
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Generation of BLNK/SLP-65-deficient mice
The cDNA for BLNK/SLP-65 was obtained by RT-PCR of RNA isolated from mouse spleens using primers 5'-AGTGGCTTGAGTTCTTGAGGC-3' and 5'-AGAAAAGCTCGTGTGAACGCC-3', and used to screen a mouse 129 genomic DNA library. Restriction enzyme digestion, Southern blotting and DNA sequencing were used to map a phage clone containing some 5' exons of BLNK. Subsequently, a targeting vector was constructed to replace the exon containing the starting ATG and a further 4.5 kb of DNA upstream with a neor gene. A 5 kb BamHIClaI fragment 5' and a 2 kb NheIBamHI fragment 3' of the deleted exon were used as the long arm and short arm of homology respectively. To inactivate BLNK in the germline, 107 E14.1 embryonic stem (ES) cells were electroporated with 10 µg of NotI-linearized targeting vector and selected with 300 µg/ml G418 (Gibco, Hong Kong, ROC) and 2 µM gancyclovir. Double-drug-resistant ES cell clones were screened by Southern blotting for homologous recombinants using probe A as shown in Fig. 1
. The frequency of targeting was 1:100. Two ES cell clones with the correct configuration of the targeted locus were injected into C57BL/6 blastocysts to generate chimeric mice for germline transmission of the mutant allele.

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Fig. 1. (A) Inactivation of BLNK/SLP-65 in the mouse germline. Partial restriction endonuclease map of the wild-type allele, the targeting vector and the inactivated allele of BLNK/SLP-65 are shown (BamHI, B; ClaI, C; EcoRI, E; KpnI, K; NheI, Nh; SacI, S; plasmid Bluescript, pBKS). The black box indicates the exon containing the starting ATG that is being replaced by the neor gene. EcoRI digestion of genomic DNA will yield fragments of 12 and 5 kb, as revealed by probe A for the wild-type and targeted alleles respectively. (B) Southern blot analysis of EcoRI-digested tail DNA obtained from wild-type, BLNK+/ and BLNK/ mice. (C) RT-PCR of bone marrow samples obtained from wild-type and BLNK/ mice. The 5' and 3' RT-PCR identified the regions corresponding to bp 38396 and 999-2013 of the SLP-65 cDNA respectively. The RT-PCR for the housekeeping gene GADPH is included as controls.
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Antibodies
The following mAb used in the flow cytometry analyses were purchased from PharMingen (San Diego, CA): anti-B220 (RA3-6B2); anti-IgM (331.12), anti-IgD (1.3-5), anti-CD43 (S7), anti-CD5 (53-7), anti-CD11b (M1/70), anti-CD23, anti-CD69, anti-CD86 (B7-2), anti-µa(DS-1) and anti-µb (AF6-78.25). The goat anti-mouse IgM F(ab)'2 fragment used in the in vitro stimulation assays was obtained from Chemicon (Temecula, CA).
FACS analyses
Tissues and cell preparations for flow cytometric analyses were prepared as previously described (16). In brief, single-cell suspensions were obtained from spleen and lymph nodes by dissociation of these tissues with a plastic mesh and a rubber-stopper from a 5 ml syringe. Peritoneal cavity and bone marrow cells were obtained by injecting staining medium (PBS containing 3% FCS and 0.1% NaN3) into the peritoneal cavity and femur and tibia respectively using a 10 and 1 ml syringe with a 26-gauge needle. All cells were treated with red blood cell lysing solution (0.15 M NH4Cl, 1 mM KHCO3 and 0.1 mM Na2EDTA) to eliminate erythrocytes. For FACS analyses, cells were stained with optimal amounts of FITC-, phycoerythrin (PE)- and biotin-conjugated mAb for 10 min on ice, and washed 3 times with staining medium. Biotin-conjugated mAb were revealed with streptavidinCyChrome. Flow cytometry analyses were performed on a FACScan (Becton Dickinson, Mountain View, CA).
In vitro stimulation and proliferation assays
Splenic B cells were obtained from wild-type and mutant mice by negative selection using MACS (Miltenyi Biotech) with anti-CD43 mAb-coupled magnetic beads that bind T cells and macrophages. The purity of B cells obtained was >90% as assessed by anti-B220 and anti-IgM mAb staining in FACS analysis. For the in vitro stimulation assay, 106 purified B cells were seeded into 48-well tissue culture plate and incubated with 10 µg/ml goat anti-mouse IgM F(ab)'2 fragment overnight in RPMI medium supplemented with 10% FCS. Cells were harvested and stained for the expression of activation markers. A colorimetric MTT assay (Roche, Singapore) was used according to the manufacturer's instructions to measure cell proliferation in vitro. Briefly, 5x105 purified B cells were stimulated with varying concentrations of goat anti-mouse IgM F(ab)'2 fragment in a 96-well tissue culture plate. After 48 h, the cells were incubated with the MTT labeling reagent for a further 4 h followed by the addition of solubilization solution overnight. Cell proliferation was quantified using an ELISA reader at 570 nm wavelength.
Immunizations of BLNK/SLP-65-deficient mice
The ability of BLNK/ mice to mount a humoral immune response was assessed by immunizing the animals with the hapten 4-hydroxy-3-nitrophenyl acetyl (NP). Wild-type and mutant mice were immunized i.p. with 10 µg NP25-Ficoll in PBS to examine their immune responses to a T cell-independent antigen. For the immune response to a T cell-dependent antigen, mice were immunized i.p. with 100 µg alum-precipitated NP17-chicken globulin (CG). Sera were obtained from mice at day 0 and 8 of immunizations to detect the presence of NP-specific antibodies in an ELISA. To detect NP-specific antibodies, the ELISA plates were coated with 50 µl of 5 µg/ml NP-BSA and blocked with 3% BSA. Pre-immune and immune sera were added at various dilutions to the wells of the ELISA plates. Specific antibodies of class IgM and IgG3 were quantified for the T-independent, and IgM and IgG1 for the T-dependent immune responses respectively.
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Results
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Generation of BLNK/SLP-65-deficient mice
BLNK/SLP-65-deficient mice were generated by deleting the exon containing the starting codon ATG and a further 4.5 kb of DNA upstream in mouse ES cells (Fig. 1
). The deletion of the exon containing the ATG was verified by Southern blotting (Fig. 1
) and by DNA sequencing (data not shown). Two targeted ES cells were injected into mouse blastocysts to generate chimera that were subsequently bred to produce mice carrying a germline mutation of BLNK/SLP-65. Homozygous mutant mice obtained were designated BLNK/. The gene targeting strategy and the derivation of homozygous mice are depicted in Fig. 1
(A and B respectively).
To ensure the inactivation of BLNK, RT-PCR was performed on bone marrow and spleen samples with primers that correspond to the 5' and 3' portions of the BLNK cDNA. As shown in Fig. 1
(C), no BLNK message was detected in the samples obtained from mutant mice compared to those from wild-type control. Thus, the BLNK loci have been disrupted.
Initial flow cytometric analyses using cell surface markers suggest that there were no detectable defects in the development of macrophages, T, NK or dendritic cells (data not shown), consistent with the fact that BLNK is not shown to be expressed in these cell types (79). The major defect of BLNK/ mice lies in the development and function of the B lineage cells, and that is the focus of our subsequent analyses.
Severe but incomplete block in B cell development in the bone marrow of BLNK/SLP-65-deficient mice
To determine the effect of BLNK/SLP-65 inactivation in early B cell development, we analyzed bone marrow cells of mutant and wild-type mice by flow cytometry. As shown in Fig. 2
(upper panel) and Table 1
, immature B220+IgM+ B cells can be found in 8-week-old mutant mice although they were reduced considerably by ~3-fold compared to wild-type control. In addition, the population of re-circulating B220highIgMlow cells was also largely diminished by 2- to 4-fold. To gain better insight into the specific B cell stage in which the BLNK/SLP-65 mutation manifests its effect, B220+IgM cells in the bone marrow were further stained with anti-CD43 mAb to resolve pro-B and pre-B cells (17). As can be seen in Fig. 2
(lower panel), BLNK/SLP-65-deficient mice lack a population of B220+CD43 pre-B cells that was reduced by 5-fold compared to wild-type animals. In addition, there was a 2-fold accumulation of B220+CD43+ pro-B cells in the bone marrow of these mutant mice. The increase in the proportion of pro-B cells in BLNK/ mice reflects an increase in the number of these cells as compared to wild-type mice (Table 1
). Thus, the inactivation of BLNK/SLP-65 results in a severe inhibition of pro-B to pre-B cell transition. However, the block in B cell development is incomplete as a small pool of IgM+ B cells is generated.

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Fig. 2. Flow cytometry analyses of bone marrow cells from wild-type and BLNK/ mice. Cells were obtained from the femur and tibia of 8-week-old mice, and stained with FITCanti-IgM, PEanti-B220 and biotinanti-CD43 (S7) mAb. The latter was revealed by streptavidinCyChrome. The upper panel depicts the B220 versus IgM staining of bone marrow cells, whereas the lower panel depicts the B220 versus CD43 profiles of IgM bone marrow cells. B cells at different stages of development are indicated. Numbers indicate percentage of cells in the lymphocyte gate. Representative of >10 analyses.
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BLNK is not required for the maintenance of peripheral B cells
Flow cytometric analyses of spleen and lymph nodes of BLNK/ mice indicate that B220+ IgM+ B cells can be found in the peripheral lymphoid tissues although they are reduced in numbers considerably (Figs 3 and 4
). This suggests that developing BLNK/ B cells can exit the bone marrow environment and seed the peripheral lymphoid organs.

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Fig. 3. Flow cytometry analysis of spleen and lymph node cells from wild-type and BLNK/ mice. (A) Spleen and lymph node cells of 3- and 12-week-old wild-type and BLNK/ mice were stained with FITCanti-IgM and PEanti-B220 mAb to resolve for the presence of B lineage cells in the periphery. Numbers indicate the percentage of cells in the lymphocyte gate. Representative of more than three analyses of mice for each age group. (B) Number of B cells found in the spleens of 3-, 7- and 12-week-old wild-type and BLNK/ mice as estimated by total splenic cell count and flow cytometry analyses as shown in (A). The fold difference in the number of B cells between wild-type and mutant mice of similar age is indicated for each age group. Analyses include more than four mice for each age group.
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Fig. 4. Severe reduction of IgMlowIgDhigh Fraction I cells in the spleen and lymph node of BLNK/ mice. Spleen and lymph node cells from 8-week-old wild-type and BLNK/ mice were stained with FITCanti-IgD and PEanti-IgM mAb to depict cells form Fractions I (IgMlowIgDhigh), II (IgMhighIgDhigh) and III (IgMhighIgDlow). Numbers indicate percentage of cells in the lymphocyte gate. Representative of more than five analyses.
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Expression of a BCR is required for the persistence of B cells in the peripheral lymphoid tissue (5). It is postulated that the BCR provides a low-level survival signal to the peripheral B lymphocytes that is distinct from the signal that is required to activate them (18). To determine whether signal transduced by BLNK is required for the maintenance of B cells in the periphery, we examine the number of B cells in the spleens of BLNK/ mice of varying age. As shown in Fig. 3
(A and B), the number of B cells that are found in 3-week-old BLNK/ mice is drastically reduced by 30-fold compared to control mice of similar age. However, as the mice grow older, the reduction in B cell numbers compared to control mice of equivalent age decreases, such that by 6 and 12 weeks of age, BLNK mutant mice have only 7- and 2-fold fewer B cells than wild-type animals of comparable age respectively. This suggests that the number of peripheral B cells in BLNK mutant mice can accumulate with age. Thus BLNK is apparently not required for the maintenance of B cells in the periphery. The accumulation of B cells in BLNK/ mice with age contrasted sharply with the situation in mb-1
c/
c mice (4) that have a truncation of the cytoplasmic tail of Ig
leading to the expression of a compromised BCR. In mb-1
c/
c mice the peripheral B cell pool remains diminished regardless of the age of the animals.
Severe reduction of IgMlowIgDhigh (Fraction I) B cells in the spleen and lymph nodes of BLNK/SLP-65-deficient mice
Peripheral B cells can be subdivided into Fractions I, II and III on the basis of differential IgM and IgD expression, and represent different stages of B cell maturation (19). Cells in Fractions III (IgMhighIgDlow) and II (IgMhighIgDhigh) are the newly emigrating or transitional B cells, whereas cells in Fraction I (IgMlowIgDhigh) are the mature B lymphocytes (20). Interestingly, as seen in Fig. 4
, most of the peripheral B cells present in the spleen of an 8-week-old BLNK/ mouse have an immature phenotype, and are found mainly in Fractions III and II. This is in contrast to wild-type mice in which the majority of the peripheral splenic B cells are found in Fraction I. This block in peripheral B cell maturation is even more evident in the lymph nodes of BLNK/ mice compared to control animals (Fig. 4
) where in the latter all cells are found in Fraction I. Thus, although BLNK/ B cells can seed the peripheral lymphoid tissues and accumulate in numbers, the majority of them do not differentiate to the IgMlowIgDhigh mature B cell stage.
Absence of CD5+ B cells in the peritoneal cavity of BLNK/SLP-65-deficient mice
Other than the conventional or B-2 cells found in the spleen and lymph nodes, another major subset of B cells, designated B-1 cells, exists, and these cells are found mainly in the pleural and peritoneal cavities. These cells can be distinguished from conventional B cells by their cell surface phenotype. In contrast to B-2 cells that express high levels of B220 and IgD, and moderate levels of IgM, B-1 cells express low levels of B220 and IgD, and high levels of surface IgM. In addition, they express CD5, a marker found on T cells, and do not express CD23 (21).
Flow cytometric analyses of 6-week-old BLNK/ mice indicate a scarcity of B cells in the peritoneal cavity of these mice compared to wild-type control (data not shown). Since B-1 cells accumulate with age, we examine the peritoneal cavity cells of 3-month-old BLNK/ mice. Detail analyses revealed that most of the cells present in BLNK/ mice are conventional or B-2 cells, with the noticeable absence of the B220lowIgMhigh and CD5+IgM+ B cells (Fig. 5
). This suggests that BLNK is required for the generation of B-1 cells.

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Fig. 5. Absence of CD5+IgM+ cells in the peritoneal cavity of BLNK/ mice. Peritoneal cavity cells were obtained from 3-month-old wild-type and BLNK/ mice and stained with FITCanti-IgM and PEanti-B220 (upper panel) or FITCanti-IgM and PEanti-CD5 (lower panel) mAb. Numbers indicate percentage of cells in the lymphocyte gate. Representative of more than five analyses.
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BLNK/SLP-65-deficient B Cells cannot be activated and do not proliferate in response to anti-IgM stimulation in vitro
Cross-linking of BCR activates B lymphocytes, resulting in their up-regulation of co-stimulatory and activation molecules. To determine whether BLNK/ B cells are functional and responsive to external stimuli, we treated purified splenic B cells from wild-type and BLNK/ mice with anti-IgM mAb in vitro. As shown in Fig. 6
(A), anti-IgM activated wild-type B cells up-regulate their expression of CD69, an early activation marker, as well as the co-stimulatory molecule, CD86 (B7-2). In contrast, BLNK/ B cells did not up-regulate either the expression of CD69 or CD86, indicating that they are non-responsive to activation via BCR cross-linking.

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Fig. 6. BLNK/ B cells cannot be activated in vitro. (A) BLNK/ B cells do not up-regulate CD86 and CD69 in response to anti-IgM stimulation. Purified splenic B cells from wild-type and BLNK/ mice were incubated in medium alone or with 10 µg/ml goat anti-mouse IgM F(ab)'2 fragment overnight, and stained with anti-B220 and anti-CD86 (B7-2) or anti-CD69 mAb. Representative of three separate experiments. (B) BLNK/ B cells do not proliferate in response to BCR cross-linking. Purified B cells from wild-type and BLNK/ mice were stimulated with increasing concentrations of goat anti-mouse IgM F(ab)'2 fragment for 48 h and cell proliferation was quantified in a MTT colorimetric assay.
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Activated wild-type B cells also undergo cell proliferation upon BCR cross-linking in a manner proportional to the concentration of stimulating anti-IgM mAb present (Fig. 6B
). However, BLNK/ B cells do not proliferate even in the presence of increasing amount of stimulant given. Thus, these data indicate that BLNK/ B cells are non-responsive to BCR cross-linking in vitro.
Impaired T cell-independent but not T cell-dependent immune responses in BLNK/ mice
Antigens that elicit an antibody response from B cells can be classified either as T independent or T dependent according to their dependency on CD4+ T cell help. To examine whether BLNK/ mice can mount an efficient immune response to exogenous antigens, we first immunized mice with NP coupled to Ficoll (NP-Ficoll), a T cell-independent antigen. The primary antibody response to NP-Ficoll is mainly of the IgM and IgG3 class. As can be seen in Fig. 7
(A), BLNK/ mice showed undetectable IgM or IgG3 antibody response to NP-Ficoll 8 days after immunization compared to the wild-type control.

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Fig. 7. BLNK/ mice have impaired immune response to T cell-independent but not T cell-dependent antigens. Groups of three wild-type ( ) and BLNK/ mice () were immunized i.p. with (A) 10 µg NP-Ficoll, a T cell-independent antigen, and (B) 100 µg alum-precipitated NP-CG, a T cell-dependent antigen. Sera were collected 8 days after immunization and quantified for the presence of NP-specific antibodies of various Ig classes in an ELISA using NP-BSA as the coating antigen. The immune sera were diluted several fold and the absorbance values for the indicated dilution (e.g. 1:100 for IgG3 in the T cell-independent immune response) were plotted. Pre-immune sera were negative for the presence of NP-specific antibodies and are not shown.
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For the T-cell-dependent immune response, we immunized mice with NP conjugated to CG (NP-CG). As shown in Fig. 7
(B) and in contrast to the situation for the T cell-independent antigen, BLNK/ mice can mount an effective immune response to NP-CG that is comparable to wild-type animals, both in terms of IgM and IgG1 secretion. Thus taken together, the data indicate that BLNK/ mice have an impaired immune response to T-independent but not T-dependent antigens.
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Discussion
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Mice deficient for the adaptor protein BLNK/SLP-65 exhibit a severe block in early B cell development at the pro-B to pre-B cell transition stage where the pre-BCR is expressed. This is consistent with the notion that a signal from the pre-BCR is required for the progression of early B lymphopoiesis (1) and presumably BLNK is needed for the transduction of such a developmental signal. However, this early developmental block is incomplete as sIgM+ B cells do develop that could eventually seed the peripheral lymphoid tissues. It is not known currently why and how these sIgM+ B cells could bypass the developmental block at the pro-B to pre-B cell transition stage. It is intriguing to speculate that perhaps these sIgM+ B cells encode for polyreactive antibodies that recognize certain environmental or self ligands with higher affinities and this heightened interaction provides the signal that could compensate for BLNK deficiency during the developmental process. This possibility can be readily tested by breeding Ig heavy and light chain transgenic mice bearing polyreactive or autoreactive antibodies with BLNK/ mice. Such experiments are in progress in the laboratory.
Interestingly, BLNK/ mice failed to generate a population of IgMlowIgDhigh B cells in the periphery and lack B-1 cells in the peritoneal cavity. In addition, BLNK/ mice could not mount an effective humoral immune response to T cell-independent antigens while maintaining a normal T cell-dependent immune response. While the current work is in progress, two other groups have also generated mice deficient in BLNK or SLP-65 (22,23). The phenotypes of the three independently generated BLNK mutant mice (22,23 and current study) are comparable and together confirmed the physiological role of BLNK in B cell development. However, we differ with respect to the inability of our BLNK/ B cells to up-regulate the expression of the activation markers CD69 and CD86 upon anti-IgM stimulation in vitro. This difference could be due to the use of an enriched population of B cell in our assay as compared to the use of total splenocytes by the other groups (22,23). It is conceivable that in the latter, other factors such as the availability of T cell help in the form of secreted cytokines might overcome the inability of BLNK/ B cells to respond to anti-IgM stimulation in vitro. Another possible explanation for the difference in our data could be the difference in the timing of assessment of the activation of BLNK/ B cells. In our study, we examine the up-regulation of the activation markers after an overnight stimulation of <18 h. Since BLNK is an adaptor molecule that facilitates the interaction of other proteins, the absence of BLNK may simply lead to a slower kinetic of activation of mutant B lymphocytes compared to wild-type cells. Indeed, further experiments will have to be conducted to determine the kinetics (if any) and parameters of activation of BLNK/ B cells in vitro. Finally, our data indicating the inability of BLNK/ B cells to proliferate and be activated by anti-IgM stimulation in vitro would correlate much better with the inability of these mutant B cells to mount a T cell-independent immune response in vivo.
It has been shown that BCR expression is required for the maintenance of peripheral B cells (5). Our additional data on the accumulation of peripheral B cells in BLNK/ mice with age suggest that signals transduced by BLNK are not involved in the persistence or maintenance of lymphocytes. This is in contrast to the situation in mb-1
c/
c mice that have a compromised BCR and in which the peripheral B cell pool does not expand with increasing age of the animals (4). These data together would imply that the cell survival signal mediated by Ig
in the BCR complex is not propagated by BLNK. Although BLNK/ B cells can accumulate in the periphery, the majority of these cells failed to mature to a IgMlowIgDhigh stage, suggesting that BLNK-transduced signal is needed for the final maturation of B lymphocytes in the secondary lymphoid tissues.
The developmental and functional defects in BLNK/ mice bear striking resemblance to xid mice that lack Btk (2426). Both mutant mice have a block in primary B lymphopoeisis, lack B-1 and mature B cells but accumulate immature IgMhighIgDlow and IgMhighIgDhigh cells in the periphery; and are unable to mount immune responses to T-independent antigens. To a lesser extent, the B cell developmental defect in BLNK/ mice is also similar to that of mutant mice lacking the tyrosine kinase Syk (27,28) and to mice with disruption of the p85
subunit of phosphoinostitide 3-kinase (PI-3K) (29,30). All these mutant mice had a block in the pro-B to pre-B cell transition and lack the IgMlowIgDhigh peripheral B cell fraction. BLNK/ mice also bear a similarity in phenotype to mice that lack the proto-oncogene Vav (3133) in that they both have increased number of IgMhighIgDlow cells and lack B-1 cells. The similarity in the phenotypes of these various mutant mice is not surprising considering that Syk, Btk, Vav, BLNK and perhaps also PI-3K could interact with each other biochemically (7,8,10,11). BLNK has been identified as the major substrate phosphorylated by Syk that leads to calcium mobilization by PLC-
2 (11). Recently, it has been shown that BLNK can also bind to the SH2 domain of Btk (10). Perhaps, it is this disruption in BtkBLNK interaction that is responsible for the lack of B-1 cells in BLNK/ mice. It remains to be established whether B-1 cells failed to be generated or, if generated, fail to be maintained in BLNK/ mice.
Btk mutation is responsible for X-linked agammaglobulinemia (XLA), a human immunodeficiency syndrome (34). A recent report indicates that mutation in BLNK can also cause human immunodeficiency (35). Since BLNK/ mice resemble xid mice, it is now of great interest to establish whether mutation in BLNK may be responsible for a large proportions of the human immunodeficiency that is not associated with a mutation in Btk. This is of particular significance as BLNK is expressed only in B cells and, unlike Syk (27,28) or PI-3K (29,30), its deficiency does not result in embryonic lethality.
Finally, disruption of SLP-76 in T cells leads to a complete block in T cell development (14,15), whereas IgM+ B cells can develop in the absence of BLNK/SLP-65 (22,23 and current study). This would suggest that although the ordered pathways for the development of T and B are quite similar, their mechanisms for the control and regulation of maturation might be quite different in some aspect (36). The availability of BLNK/ mice will no doubt aid in the further study of the B cell differentiation process.
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Acknowledgments
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We thank Dr Leonore Herzenberg for advice, Edwin Oh and Siew-Cheng Wong for insight discussion, and the In Vivo Model Unit of IMCB for the care and maintenance of mice. This work is supported by grants from The National Science and Technology Board (NSTB) of Singapore.
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Abbreviations
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BCR B cell receptor |
BLNK B cell linker protein |
Btk Bruton's tyrosine kinase |
CG chicken globulin |
ES embryonic stem cell |
NP 4-hydroxy-3-nitrophenyl acetyl |
PI-3K phosphoinostitide 3-kinase |
PLC phospholipase C |
SLP SH2 domain-containing leukocyte protein |
xid X-linked immunodeficiency |
XLA X-linked agammaglobulinemia |
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Notes
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Transmitting editor: D. Tarlinton
Received 6 December 1999,
accepted 3 January 2000.
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