A clone of murine IL-3-dependent BaF3 cells transfected with a BCR/ABL cDNA under the control of a tetracycline-inducible promoter, Ton.B210 and the parental control clone, Ton.BaF, were kindly provided by Dr G. Daley (23). Ton.B210 cells were cultured in 10% fetal calf serum (FCS) containing RPMI-1640 medium supplemented either with 10% Wehi3B conditioned medium as the source of IL-3 or with 1 μg/ml doxycycline, which induces the expression of BCR/ABL. Ton.B210/E255K or Ton.B210/T315I cells (16), which inducibly express BCR/ABL with the E255K or T315I mutation, respectively, and 32Dcl3 cells expressing BCR/ABL, Ton.32Dp210 (17), were described previously. The human CML cell line K562 was obtained from the Riken Cell Bank (Ibaraki, Japan). TMD-5 cells, a double Ph⁺ ALL-derived cell line expressing the p190 form of BCR/ABL, were kindly provided by Dr S. Tohda (24). Leukemic blasts were isolated from patients with CML myeloid crisis, Ph⁺ ALL, or Ph⁺ biphenotypic acute leukemia as described previously (16). Written informed consent was provided according to the Declaration of Helsinki, and the study was approved by the ethics committee of Tokyo Medical and Dental University. PLAT-A (25), an amphotropic virus packaging cell line, and 293T (26), a human embryonic kidney cell line, were kindly provided by Dr T. Kitamura and Dr S. Yamaoka, respectively, and maintained in Dulbecco’s modified Eagle’s medium (DMEM) supplemented with 10% FCS.

Imatinib was kindly provided by Novartis (Basel, Switzerland). Dasatinib and sorafenib were purchased from Toronto Research Chemicals Inc. (Toronto, Canada) and LKT Laboratories (St. Paul, MN), respectively. Doxycycline and fibronectin were from Calbiochem (San Diego, CA) and Gibco-BRL (Grand Island, NY), respectively. DiOC₆ was purchased from Invitrogen (Carlsbad, CA).

Antibodies against PECAM-1 (SC1506), Lyn (SC15), CrkL (SC319), SHP2 (SC280), BCR (SC885), and phospho-Y694-STAT5 (SC9359) were purchased from Santa Cruz Biotechnology (Santa Cruz, CA). An anti-phosphotyrosine monoclonal antibody (4G10, 05-321) as well as antibody against Gab2 (06-967) was purchased from Millipore (Billerica, MA). Antibodies against phospho-Y416-Src (9359) and cleaved caspase-3 (9661) were purchased from Cell Signaling Technology (Beverly, MA). Antibodies against phospho-Y396-Lyn (1645) and β-actin were purchased from Epitomics Inc. (Burlingame, CA) and Sigma, respectively.

Expression plasmids for BCR/ABL, pcDNA3-BCR/ABL, and that for the 56-kDa form of Lyn, pXM-LynA, were described previously (27,28). Retrovirus vectors, pRevTRE and pMIG (Addgene plasmid 9044), were obtained from Clontech (Palo Alto, CA) and Addgene (Cambridge, MA), respectively. pMXs-IG (29) was kindly provided by Dr T. Kitamura. Expression plasmids for wild-type PECAM-1 and its mutant with Y663F and Y686F mutations in the ITIM motives, PECAM-1-ITIM (−), in pcDNA3.0 vector were kindly provided by Dr D. Newman (30,31). The coding regions for wild-type and mutant PECAM-1 were subcloned from these plasmids into retroviral vectors pREV-TRE (HindIII/EcoRV), pMIG (EcoRI) and pXMs-IG (EcoRI) using the restriction enzymes in parentheses. Expression plasmids for wild-type and substrate-trapping mutant of SHP2, pIRES2-EGF-SHP2-Wt and -DA (Addgene plasmids 12283 and 12286) (32), respectively, were obtained from Addgene. The coding sequences for SHP2-Wt and -DA were excised from these plasmids using XhoI and SmaI and subcloned into pREV-TRE to give pREV-SHP2-Wt and -DA. An expression plasmid for BCR/ABL, pTetP210, was kindly provided by Dr G. Daley (23). The coding sequence for BCR/ABL was excised from pTetP210 using EcoRI and subcloned into pRxZiN obtained from the Riken Gene Bank to give pRxP210.

For transient expression in 293T cells, cells were transfected with indicated plasmids using the Lipofectamine reagent (Invitrogen) according to the manufacturer’s instructions. Cells were harvested 48 h after transfection for immunoprecipitation and immunoblotting.

To obtain BaF3 cells constitutively expressing BCR/ABL, Ton.BaF cells were infected with the recombinant retrovirus obtained from PLAT-A transfected with pRxP210, as described previously (33). Infected cells were cultured in medium lacking IL-3, and a clone expressing BCR/ABL at a high level was selected by limited dilution to give Ton.Bp210-8. This cell line was subsequently transduced again with pRev-PECAM-1, -ITIM (−), or pRevTRE and selected in medium containing hygromycin. Cells were used for subsequent experiments after expression of PECAM-1 or PECAM-1-ITIM (−) was confirmed by immunoblotting. To obtain Ton.B210 cells overexpressing wild-type SHP2 or the D425A mutant, Ton.B210 cells were transduced with pRev-SHP2-Wt or -DA, respectively, and selected in medium containing hygromycin. To obtain Ton.32Dp210 or K562 cells overexpressing PECAM-1 or PECAM-1-ITIM (−), these cells were transduced by the retrovirus vectors in pMXs-IG for pMIG, as described above. GFP-positive cells were sorted by flow cytometry, and expression of PECAM-1 or its mutant as well as BCR/ABL was confirmed by immunoblotting.

Cells were lysed and subjected to immunoprecipitation and immunoblotting as described previously (34). The results shown are representative of experiments repeated at least three times.

Cell viability was assessed by counting viable and non-viable cell numbers by the trypan blue dye exclusion method. Flow cytometric analysis of cell cycle and apoptosis was performed as described previously (16). Flow cytometric analysis of caspase-3 cleavage was performed using specific antibodies against cleaved caspase-3 as described previously (17). For analysis of Δψ_m, cells were stained with DiOC₆ (Invitrogen) and analyzed by flow cytometry as described previously (16).

Adhesion assays were performed essentially as described previously (35,36). In brief, cells were labeled with 5 μM BCECF/AM (Dojindo, Kumamoto, Japan) and plated on wells coated with 5 μg/ml fibronectin for 30 min at 37°C. Adherent cells were measured by Cytofluor II fluorescent plate reader (PerSeptive Biosystems, Foster City, CA). After subtraction of background cell binding to bovine serum albumin-coated wells, the percentage of adherent cells was determined by dividing the fluorescence intensity of the adherent cells by that of the initial cell input.

To examine possible involvement of PECAM-1 in BCR/ABL-mediated signaling, we first examined whether it is tyrosine phosphorylated in primary Ph⁺ leukemic cells. As shown in Fig. 1A, PECAM-1 was conspicuously phosphorylated on tyrosine in Ph⁺ biphenotypic acute leukemia or ALL cells, which was mostly abolished by treatment with the tyrosine kinase inhibitor imatinib or dasatinib. Essentially the same results were obtained with primary leukemic cells from another patient with Ph⁺ ALL expressing the p190 form of BCR/ABL and a patient with CML in myeloid blastic crisis expressing the p210 form of BCR/ABL (Fig. 1B and C, respectively). We also examined a Ph⁺ ALL cell line expressing the p190 form of BCR/ABL, TMD-5, and found that PECAM-1 was also tyrosine phosphorylated in these cells and was dephosphorylated after treatment with imatinib (Fig. 1D and E). These results suggest that PECAM-1 is a substrate of both p190 and p210 forms of BCR/ABL in these leukemic cells.

We next examined murine model hematopoietic cell lines 32Dcl3 and BaF3 engineered to express BCR/ABL. As shown in Fig. 2A and B, PECAM-1 was tyrosine phosphorylated also in these cells, which was completely dephosphorylated by dasatinib. However, imatinib only partially inhibited tyrosine phosphorylation of PECAM-1 in these cells. Because dasatinib, but not imatinib, also inhibits the Src family tyrosine kinases in addition to BCR/ABL, we examined the activation specific tyrosine phosphorylation of these kinases. As shown in Fig. 2C, western blot analysis with an antibody specific for Lyn activation showed that imatinib drastically inhibited activation of Lyn in BCR/ABL-expressing BaF3 cells. However, examination with an antibody that detects activation of the various Src family kinases revealed that some of the activated kinases were resistant to imatinib (Fig. 2C). On the other hand, dasatinib strongly inhibited activation of the Src family kinases including Lyn. These data suggest that Lyn is activated by BCR/ABL in these cells, while some of the other Src family members are constitutively activated independent of BCR/ABL. We also examined the well-established BCR/ABL substrates STAT5 and CrkL in these cells (12). Similar to PECAM-1, tyrosine phosphorylation of CrkL, which was examined by the mobility shift assay, was also abrogated by dasatinib but only partially inhibited by imatinib (Fig. 2C). By contrast, imatinib abrogated tyrosine phosphorylation of STAT5 in BaF3 cells expressing BCR/ABL. These results suggest that the tyrosine phospho rylation of PECAM-1 as well as CrkL, but not that of STAT5, is mediated at least partly by the Src family kinases activated independent of BCR/ABL in these cells.

We next examined the possibility that tyrosine phospho rylated PECAM-1 is a substrate for the SHP2 tyrosine phosphatase in these cells, because SHP2 forms a physical complex with tyrosine phosphorylated PECAM-1 in various types of cells (4,37). For this purpose, we overexpressed wild-type SHP2 or its dominant-negative, substrate-trapping mutant SHP-2-D425A (7,32,38) in Ton.B210 cells. As shown in Fig. 2D and E, overexpression of SHP2-D425A, but not wild-type SHP2, profoundly enhanced tyrosine phosphorylation of PECAM-1 and SHP2. Although SHP2 was found to form a complex with PECAM-1 as well as Gab2 in these cells, tyrosine phosphorylation of PECAM-1, but not that of Gab2, that was associated with SHP2 was drastically enhanced by overexpression of SHP2-D425A (Fig. 2E). Tyrosine phosphorylation of SHP2 was also prominently increased in SHP-2-D425A-expressing Ton.B210 cells. These results suggest that PECAM-1 is a major binding partner and substrate of SHP2 in BCR/ABL-expressing cells.

To examine further the mechanisms of tyrosine phosphorylation of PECAM-1 induced by BCR/ABL, we next examined it in transiently transfected 293T cells. As shown in Fig. 3A, co-expression of BCR/ABL induced tyrosine phosphorylation of wild-type PECAM-1 but not that of PECAM-1-ITIM (−) with the mutated ITIM motives (Y663F, Y686F), thus indicating that BCR/ABL induces tyrosine phosphorylation of one or both of these ITIM motives. In accordance with a previous report (39), a smaller 120-kDa form of PECAM-1, which most likely represents a differently glycosylated form, was unambiguously observed in transfected cells.

Because Lyn was activated by BCR/ABL and the Src family kinases were implicated in induction of tyrosine phosphorylation of PECAM-1 in BaF3 cells (Fig. 2B and C), we next examined the ability of Lyn to phosphorylate PECAM-1. When co-expressed in 293T cells, Lyn induced a robust tyrosine phosphorylation of PECAM-1, which was more conspicuously observed than that induced by BCR/ABL (Fig. 3B and C). Lyn also failed to induce phosphorylation of PECAM-1-ITIM (−). These results are consistent with the idea that the Src kinases including Lyn may partly mediate tyrosine phosphorylation of PECAM-1 on the ITIM motives in cells expressing BCR/ABL.

E255K and T315I are the most predominant mutations of BCR/ABL causing imatinib resistance in patients and may increase the kinase activity or change the substrate preferences of BCR/ABL (15,18). Thus, we next examined tyrosine phosphorylation of PECAM-1 in cells expressing BCR/ABL harboring these mutations. As shown in Fig. 4A, PECAM-1 was more prominently tyrosine phosphorylated in BaF3 cells expressing the E255K or T315I mutant as compared with cells expressing native BCR/ABL. Moreover, as shown in Fig. 4B, SHP2 physically associated with PECAM-1 more prominently in cells expressing the E255K or T315I mutant as compared with cells expressing native BCR/ABL, while these mutants had less significant effects on complex formation between SHP2 and Gab2. Tyrosine phosphorylation of STAT5 was also enhanced, though not as significantly as that of PECAM-1, in cells expressing the E255K or T315I mutant (Fig. 4C).

We next examined the effect of dasatinib on tyrosine phosphorylation of PECAM-1 in BaF3 cells expressing the T315I mutant, which is totally resistant to dasatinib as well as imatinib but sensitive to the multi-kinase inhibitor sorafenib (17,22). As shown in Fig. 4D, dasatinib or sorafenib partially inhibited tyrosine phosphorylation of PECAM-1. It was confirmed that sorafenib, in contrast to dasatinib, showed inhibitory effect on autophosphorylation of BCR/ABL or phosphorylation of its substrate STAT5 in these cells (Fig. 4E), thus indicating it partially inhibited the T315I mutant in these cells. In 293T cells, the T315I mutant also induced tyrosine phosphorylation of PECAM-1 much more prominently than native BCR/ABL, which was abolished by sorafenib but not affected by dasatinib and correlated with autophosphorylation of BCR/ABL (Fig. 4F and G). The increase in autophosphorylation of the T315I mutation as compared with native BCR/ABL was not so prominent as compared with that in PECAM-1 phosphorylation. These results suggest that the tyrosine phosphorylation of PECAM-1 is mediated both directly by the T315I BCR/ABL mutant and by the Src family kinases in BaF3 cells and exclusively by BCR/ABL in 293T cells.

To examine the cellular effects of PECAM-1 in Ph⁺ leukemic cells, we next examined the human CML K562 cell line, which expresses endogenous PECAM-1 at a barely detectable level (Fig. 5A). As in other BCR/ABL-expressing cells, PECAM-1 overexpressed in K562 cells was tyrosine phosphorylated, which was moderately inhibited or abolished by imatinib or dasatinib, respectively (Fig. 5B). On the other hand, K562 cells overexpressing PECAM-1-ITIM (−) showed a very low level of PECAM-1 phosphorylation, thus suggesting that the ITIM motives are mainly tyrosine phosphorylated also in these Ph⁺ leukemic cells.

We first examined the possible effect of PECAM-1 on cell adhesion. As shown in Fig. 5C, adhesion of K562 to fibronectin-coated plate was enhanced by overexpression of PECAM-1 or PECAM-1-ITIM (−). These data are in agreement with the previous reports that PECAM-1 may play a role in regulation of integrin activation and cell adhesion in various cell types (3,37).

We next examined the possibility that PECAM-1 may affect the sensitivity of Ph⁺ leukemic cells to the tyrosine kinase inhibitors, because PECAM-1 has been implicated in prevention of apoptosis in various types of cells (40–44). As shown in Fig. 6A and B, the decline in viability induced by imatinib was downregulated by overexpression of PECAM-1 or, to a lesser degree, by that of PECAM-1-ITIM (−) in BCR/ABL-expressing 32D cells or in K562 cells, respectively. Moreover, PECAM-1 or its mutant was found to partially prevent depolarization of Δψ_m in K562 cells treated with imatinib or dasatinib (Fig. 6C). In accordance with this, PECAM-1 also partially protected K562 cells from imatinib-induced cleavage of caspase-3 (Fig. 6D). It was finally confirmed that PECAM-1 or its mutant decreased the number of K562 cells with sub-G1 DNA content, a hallmark of cells undergoing apoptosis, after treatment with imatinib (Fig. 6E). Similarly, overexpression of PECAM-1 or its mutant in 32D cells partially downregulated depolarization of Δψ_m, cleavage of caspase-3, and appearance of cells with sub-G1 DNA content induced by imatinib (data not shown). Overexpression of PECAM-1 and its mutant showed comparable anti-apoptotic effects in these repeated experiments in K562 and 32D cells. These data suggest that PECAM-1 may partially protect BCR/ABL-expressing leukemic cells treated with the tyrosine kinase inhibitors from activation of mitochondria-mediated apoptotic pathway leading to caspase activation and DNA fragmentation, at least partly, in an ITIM-independent manner.