The proteasome inhibitor bortezomib affects osteoblast differentiation in vitro and in vivo in multiple myeloma patients

doi:10.1182/blood-2006-11-059188

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Blood, 1 July 2007, Vol. 110, No. 1, pp. 334-338.
Prepublished online as a Blood First Edition Paper on March 19, 2007; DOI 10.1182/blood-2006-11-059188.

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NEOPLASIA
The proteasome inhibitor bortezomib affects osteoblast differentiation in vitro and in vivo in multiple myeloma patients
Nicola Giuliani¹, Francesca Morandi¹, Sara Tagliaferri¹, Mirca Lazzaretti², Sabrina Bonomini¹, Monica Crugnola¹, Cristina Mancini², Eugenia Martella², Luca Ferrari¹, Antonio Tabilio³, and Vittorio Rizzoli¹
¹ Hematology and Bone Marrow Transplantation Center, Department of Internal Medicine and Biomedical Science, University of Parma, Italy; ² Pathology, University of Parma, Italy; ³ Department of Internal Medicine and Public Health, University of Chieti, Italy

   Abstract

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
Authorship
References

The proteasome inhibitor bortezomib may increase osteoblast-relatedmarkers in multiple myeloma (MM) patients; however, its potentialosteoblastic stimulatory effect is not known. In this study,we show that bortezomib significantly induced a stimulatoryeffect on osteoblast markers in human mesenchymal cells withoutaffecting the number of osteoblast progenitors in bone marrowcultures or the viability of mature osteoblasts. Consistentlywe found that bortezomib significantly increased the transcriptionfactor Runx2/Cbfa1 activity in human osteoblast progenitorsand osteoblasts without affecting nuclear and cytoplasmaticactive ß-catenin levels. Consequently a stimulatoryeffect of bortezomib on bone nodule formation was also demonstratedin osteoblast progenitors. These in vitro observations wereconfirmed in vivo by the finding of a significant increase inthe number of osteoblastic cells x mm² of bone tissue and inthe number of Runx2/Cbfa1-positive osteoblastic cells that wasobserved in MM patients who responded to bortezomib. Our invitro and in vivo observations support the hypothesis that adirect stimulatory effect on bone formation process could occurduring bortezomib treatment.

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
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Multiple myeloma (MM) is a plasma cell malignancy characterizedby the high capacity to induce osteolytic bone lesions.¹ Hystomorphometricstudies showed that osteoblast formation and function are profoundlyimpaired in MM patients and critical in the bone lesion development.^1–3Several mechanisms are involved in MM-induced osteoblast suppression^1,4,7including the production of Wnt inhibitors as DKK-1 or sFRP-2^5,6or the impairment of osteoblast formation and differentiationthrough the block of the critical osteoblast transcription factorRunx2/Cbfa1.⁷ In turn, osteoblastic cells also regulate myelomacell growth^8,9 and the increase of bone formation in mice resultsin a reduction of tumoral burden.¹⁰
Recent data suggest that ubiquitin-proteasome pathway, whichis the major cellular degradative system and therapeutic targetin myeloma cells,¹¹ also regulates osteoblast differentiation.^12–14The ubiquitin-proteasome pathway can modulate the BMP-2 expression,¹²which can induce osteoblast differentiation through the Wntsignaling¹³ and regulates the proteolytic degradation of theosteoblast transcription factor Runx2/Cbfa1.¹⁴ Recently, Garrettet al¹² demonstrated that proteasome inhibitors as PS1 and epoximicinstimulate bone formation in neonatal murine calvarial bonesand in vivo in mice.¹² A strong correlation between the capacityof these compounds to inhibit proteasomal activity in osteoblastsand their bone-forming activity was also demonstrated.¹² Preliminaryobservations obtained in MM patients treated with the proteasomeinhibitor bortezomib show an increase of serum bone-specificalkaline phosphatase and other osteoblast related markers suggestinga potential osteoblast stimulatory effect of this drug.^15–18Currently it is not known whether the proteasome inhibitor bortezomibmay have a direct effect on osteoblast differentiation and formationin vitro in human cultures and in vivo in MM patients.

   Patients, materials, and methods

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Introduction
Patients, materials, and methods
Results
Discussion
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References

Drugs
Bortezomib was purchased from Janssen-Cilag (Milan, Italy).For in vitro studies, the drug was reconstituted in DMSO ata stock concentration of 50 mM, and this stock was diluted inmedium just before use, so that the concentration of DMSO neverexceeded 0.1%. The proteasome inhibitors MG-132 and MG-262 werepurchased from BIOMOL International (Plymouth Meeting, PA; DBAsrl, Milan, Italy).
Cells and cell culture conditions
Isolated human BM mononuclear cells were seeded in 6-well platesat the density of 10⁶/well in 4 mL ${alpha}$ -MEM medium with 15% of FCS,plus ascorbic acid (50 µg/mL) and dexamethasone (Dex)(10^–8M) and incubated in the presence or absence of bortezomib(concentration ranging from 2 nM to 5 nM) for 2 to 3 weeks replacingthe medium every 3 days. Colonies forming units–fibroblast(CFU-Fs) and CFU-osteoblasts (OBs) were evaluated by alkalinephosphatase and alizarin red (Sigma Aldrich, St Louis, MO) stainingand quantified as previously described.⁷
Human trabecular SV-40–transfected osteoblasts (HOBITs)(Dr Riggs, Mayo Clinic, Rochester, MN) or osteoblast-like cellsMG-63 (DSM, Braunschweig, Germany) or human BM osteoprogenitorcells (PreOBs) obtained from mesenchymal cells as previouslydescribed.⁷ Cells (2 x 10⁶) were incubated in the presence orabsence of bortezomib (2 nM to 5 nM) or PTH (1-34) (PhoenixPharmaceutical, Belmont, CA) at 50 ng/mL or BMP-2 (Peprotech,London, United Kingdom) at 50 ng/mL or MG-132 (10-100 nM) orMG-262 (10 nM) for 24 to 48 hours. Cell viability and survivalwere assessed as previously described.⁷ In parallel experiments,confluent PreOBs were incubated in the presence or absence ofbortezomib (2-5 nM) or BMP-2 (50 ng/mL) or PTH (1-34) (50 ng/mL)or MG-132 (100 nM) or MG-262 (10 nM) for 21 days in ${alpha}$ -MEM mediumwith 15% of FCS plus ascorbic acid (50 µg/mL), Dex (10^–8M) and ß-glycerophosphate 10 mM. At the end of cultureperiod, the cells were fixed with 1:1 mixture (vol/vol) of 37%formaldehyde and ethanol for 5 minutes, washed 3 times withPBS, and stained for 10 minutes with a solution of 2% of alizarinred (Sigma Aldrich) at pH 4.2. Bone nodules were quantifiedby light microscopy as previously described.⁷ Images were visualizedunder an Eclipse TE 300 microscope with a digital DS-UI slight(Nikon Instruments, Florence, Italy). Image processing was performedwith Adobe Photoshop 5.02.
RNA isolation and reverse transcriptase-polymerase chain reaction amplification
Reverse transcriptase-polymerase chain reaction (RT-PCR) analysiswas performed as previously described.⁷ cDNAs were amplifiedby PCR using specific primer pairs for human Runx2/Cbfa1, collagenI, osteocalcin (OC), alkaline phosphatase (ALP), and ß-catenin.⁷PCR reactions were performed in a thermal cycler (MiniCycler;MyResearch, Watertown, MA) for 30 cycles.
Western blot analysis
Nuclear and cytosolic extracts were obtained using a commercialkit (Active Motif, Carlsbad, CA). Polyclonal anti–collagenI and anti-Runx2/Cbfa1 (Santa Cruz Biotechnology, Santa Cruz,CA) were used as primary Abs. ß-Catenin protein expressionwas checked using anti–ß-catenin mAb recognizingthe active dephospho nuclear form (aa 27-37) (Alexis Biochemicals,San Diego, CA), or anti–ß-catenin mAb recognizingthe inactive phospho form (pSer⁴⁵) (Sigma, St Louis, MO). Asinternal controls, anti–ß-actin (Sigma) andanti–Histone H1 mAbs (Upstate, Lake Placid, NY) were usedfor cytosol lysates and nuclear ones, respectively. Immunoblotprocedures were performed as previously described.⁷
Runx2/Cbfa1 binding activity
Runx2/Cbfa1 binding activity was assessed by an enzyme-linkedimmunosorbent assay (ELISA)–based assay as previouslydescribed¹⁹ (TransAM Runx2; Active Motif, Vinci Biochem, Florence,Italy) according to the manufacturer's procedures. Nuclear extractsof human cell lines Saos2 with or without wild-type (WT) ormutated (MT) consensus-specific oligonucleotides were testedas controls for Runx2 activity.
Patients and treatment schedule
MM patients (n = 21) included in the study were at least 18years old (median age, 72 years; range, 58–86 years),stages I to III, had measurable relapse, had at least 2 linesof therapy and/or refractory myeloma, and had BM plasmacytosismore than 30%. Fourteen of 21 patients have osteolytic lesionsand previously underwent bisphosphonate therapy with zoledronicacid. Other inclusion criteria were similar to those previouslyreported.²⁰
Bortezomib (1.3 mg/m²) was administered in monotherapy by intravenousbolus on days 1, 4, 8, and 11 of a 21-day cycle for up to 8cycles. Patients with a suboptimal response, defined as progressivedisease after 2 cycles or no change after the first 4 cyclesof bortezomib, could receive oral dexamethasone (20 mg) on thesame day and the day after bortezomib treatment. Responses werecategorized as previously reported.² All patients provided writteninformed consent in accordance with the Declaration of Helsinki.Our study was approved by our local ethics committee, "AziendaOspedaliero-Universitaria di Parma," Parma, Italy.
ELISA
Soluble osteocalcin levels in cell-conditioned media were detectedusing an ELISA assay purchased from Nordic Biosciences Diagnostic(Herlev, Denmark). The serum C-terminal telopeptides of collagenI (CTX) were measured in the peripheral serum of MM patientsusing the Serum CrossLaps ELISA kit from Nordic BiosciencesDiagnostic.
Immunohistochemistry
Immunohistochemical staining was performed on 3-µm-thickBM sections obtained from the 21 MM patients before and after8 cycles of bortezomib treatment with goat anti-Runx2/Cbfa1Ab (Santa Cruz Biotechnology) using the immunoperoxidase techniqueas previously described.⁷ Normal bones obtained from 5 subjectswithout hematologic or bone disease were used as control. Thetotal trabecular area of each section was measured by a dedicatedsoftware analyzer (Image Pro Plus 4.5, Media Cybernetics, SilverSpring, MD). Osteoblastic cells were identified in BM biopsiesusing morphologic criteria, as previously described.^2,3,7 Osteoidsurface was evaluated in Goldner trichrome-stained section (Olympus8 x 60 F5 microscope equipped with a Uplan Fi 100x/1.30 iris,WH 10 x 22; Olympus, Tokyo, Japan). An Olympus oil DP10 digitalmicroscope camera system was used for image acquisition. Imageswere processed by Adobe Photoshop 5.02.

   Results

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Effect of bortezomib on the number of osteoblast progenitors in human BM culture and on mature osteoblasts
In human BM cultures, we found that bortezomib in a wide rangeof concentration did not significantly reduce the number ofboth early bone marrow (BM) osteoblast progenitors CFU-F andlate CFU-OBs (Figure 1A). Similarly, we found that bortezomibdid not inhibit the proliferation and survival (Figure 1B) ofosteoblastic cell lines HOBIT and MG-63 at concentrations rangingfrom 2 nM to 5 nM that are known to be subapoptotic or apoptoticfor human myeloma cells,²¹ indicating that long-term treatmentwith bortezomib did not show any toxic effect on osteoblastand the osteoblastogenesis process.

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Figure 1. Effect of bortezomib on osteoblast progenitors and osteoblastic cells. Colony-forming units–fibroblast (CFU-Fs) and CFU-osteoblasts (OBs) were evaluated by alkaline phosphatase and alizarin red staining, respectively, in long-term human BM cell cultures incubated in the presence or absence of bortezomib at a concentration ranging from 2 nM to 5 nM (A). Human osteoblastic cells MG-63 or HOBITs (2 x 10⁶) were incubated in the presence or absence of bortezomib (2 nM to 5 nM) for 48 hours. The number of dead and apoptotic osteoblastic cells was evaluated by a colorimetric method. Osteoblastic cells treated with TRAIL or stimulating anti-CD95 Ab (FAS) have been used as positive control (CON = control) (B). mRNA expression of the osteoblast-related markers was evaluated by RT-PCR in human PreOBs treated with bortezomib or vehicle for 24 hours (C). PreOBs were treated with bortezomib or vehicle for 48 hours; thereafter, collagen I and Runx2/Cbfa1 protein expression was evaluated by Western blot analysis in cell lysates and osteocalcin (OC) levels detected in conditioned media by ELISA. Graphs represent the mean OCs ± SD of 3 repeated experiments measured twice (D). The activity of the transcription factor Runx2/Cbfa1 was evaluated by an ELISA-based method in nuclear lysates of PreOBs and HOBITs treated for 48 hours with bortezomib (2-5 nM). Graphs represent the mean Runx2/Cbfa1 activation ± SD using 10 µg protein in 3 repeated experiments measured in triplicate (E). Both dephospho and phospho ß-catenin were determined by Western blot in cytosolic or nuclear lysates of PreOBs treated with bortezomib (2-5 nM) or vehicle. Actin and histone H1 were used as internal controls (F).

Effect of bortezomib on osteogenic differentiation of human osteoprogenitor cells
In short-term experiments, we found that 24-hour bortezomib(2-3 nM) treatment increased mRNA expression of the osteoblastmarkers collagen I and OC but not ALP, Runx2/Cbfa1, and ß-catenin(Figure 1C) by human PreOBs. Collagen I production and OC secretionby PreOBs have been stimulated after 48 hours of bortezomibtreatment without modifying Runx2/Cbfa1 protein level (Figure 1D).On the other hand, bortezomib did not have any effect on ALPactivity in PreOBs (data not shown). Consistently with theseobservations, we found that bortezomib at low concentrationsignificantly increased the activity of the transcription factorRunx2/Cbfa1 both in PreOBs and HOBITs (Figure 1E). On the otherhand, bortezomib (2-5 nM) did not have any effect on activedephospho ß-catenin cytosolic and nuclear levels oron inactive phosphorylated ones in PreOBs (Figure 1F) and HOBITs(data not shown), suggesting that bortezomib did not affectcanonical Wnt signaling in these cells.
Thereafter, the effect of bortezomib was compared with thoseobserved with BMP-2 and PTH (1-34) as well as with the specificproteasome inhibitors MG-132 and MG-262. A stimulatory effectof all these compounds was observed after short-term expositionon collagen I expression without affecting Runx2/CBFA1 mRNAexpression (Figure 2A).

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Figure 2. Effect of bortezomib on osteogenic differentiation of human mesenchymal cells. Confluent PreOB cells were treated with or without bortezomib (2 nM) or BMP-2 (50 ng/mL) or PTH (1-34) (50 ng/mL) or MG-132 (100 nM) or MG-262 (10 nM). After 24 hours, collagen I, Runx2/Cbfa1, and GAPDH mRNA expression was evaluated by RT-PCR (A). Adherent PreOB cells were incubated in osteogenic differentiating medium as described in "Patients, materials, and methods" in the presence or absence of bortezomib (2 nM) or BMP-2 (50 ng/mL) or PTH (1-34) (50 ng/mL) or MG-132 (100 nM) or MG-262 (10 nM) for 21 days, replacing medium with fresh one every 3 days. After the culture period, cells were fixed and stained for the presence of bone nodules by alizarin red. Graphs and bars represent the mean plus SD of bone nodules x field of 2 independent experiments performed in triplicate (*P < .05; **P < .01) (B). Images were obtained on a Nikon Eclipse TE 300 microscope at 10x/0.13 using a DS-U1 digital slight and at 4x/0.12 objective lens (Original magnification x 5).

Then the potential effect of bortezomib on calcium depositionin adherent PreOBs has been evaluated in comparison with BMP-2,PTH, (1-34) MG-132, and MG-262. As shown in Figure 2, we foundthat bortezomib significantly increased bone nodule formationafter 21 days of exposition. Both BMP-2 and PTH (1-34) had amore potent effect on calcium deposition by PreOBs, whereasMG-132 and MG-262 showed a similar stimulatory effect on bonenodule formation by PreOBs in comparison with bortezomib (Figure 2B).
Effect of bortezomib on osteoblastic cells, bone formation rate, and bone resorption in MM patients
To put our in vitro observations in a clinical perspective,we evaluate the potential in vivo effect of bortezomib in acohort of MM patients. A significant increase in the numberof osteoblastic cells x mm² of bone tissue was observed in MMpatients responding to bortezomib treatment (complete remission[CR], near complete remission [nCR], and partial remission [PR])but not in nonresponders (Figure 3A). However, the number ofosteoblastic cells x mm² of bone tissue in responder MM patientsafter therapy was still decreased compared with healthy boneobtained from the control group (Figure 3A). Finally, we founda significant increase in the number of Runx2/Cbfa1-positiveosteoblastic cells in responder MM patients compared with nonresponders(Figure 3A-B). Consequently, an increase of osteoid surfacewas observed in the area with higher number of osteoblasts afterbortezomib treatment in responders as shown for a representativepatient (Figure 3B).

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Figure 3. Effect of bortezomib on bone formation in MM patients. Histomorphometry and Runx2/Cbfa1 immunostaining performed on BM biopsies of 21 MM patients before and after 6 to 8 cycles of bortezomib in monotherapy according to the schedule described in the "Patients, materials, and methods." The graphs and bars represent the mean plus SD of the number of osteoblasts (OBs)/mm² and the percentage of Runx2/Cbfa1-positive OBs (A). Runx2/Cbfa1 immunostaining performed in a trabecula of 2 representative MM patients who responded or not to bortezomib treatment (original magnification, x 200; small insert, x 400) (B). Goldner trichrome–stained sections from a representative MM responder patient. (Microscope used was an Olympus B x 60 F5 equipped with a UPlan F: 100x/1.30 oil iris, WH10x/22. An Olympus DP10 digital microscope camera system was used for image acquisition (original magnification, x 200) (C).

Osteoclast activity was also evaluated in our cohort of patientsby the measure of serum CTX levels. A reduction of serum CTXwas observed in MM patients treated with bortezomib even ifit did not reach a statistical significance either in nonresponderor responder patients (Figure 4).

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Figure 4. Serum CTX in MM patients before and after bortezomib. Serum CTX was measured by ELISA assay in 21 MM patients before and after bortezomib treatment. Box plots represent the median CTX serum levels with the 25th to 75th percentiles.

   Discussion

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Emerging data indicate that the proteasome inhibitors may havea critical role in the regulation of osteoblast proliferationand differentiation in murine system.^12–14 In this study,we show that bortezomib, the first member of this class of drugsapproved for the clinical use, affects human osteoblast differentiationprocess both in vitro and in vivo.
It is known that human osteoblastogenesis is primarily associatedwith increased Runx2/Cbfa1 activity without a change in mRNAor protein level.²² The binding sites of Runx2/Cbfa1 have beenidentified in the major bone matrix genes as collagen I andOC and its activation induced the expression of these genesor activated their promoters in vitro.²³ Our data suggest thatbortezomib may induce osteoblast phenotype in osteoblast progenitorsincreasing Runx2/Cbfa1 activity without changing Runx2/Cbfa1mRNA level and consequently stimulating the expression of lateosteoblast markers as collagen I and OC rather than the earlyones as ALP. On the other hand, we failed to find a stimulatoryeffect on the canonical Wnt signaling. Accordingly, it has beenreported that Wnt/ß-catenin signaling induces ALPexpression, but has no effect on OC and collagen I expressionby osteoprogenitor cells.^13,24 The stimulatory effect of bortezomibon Runx2/Cbfa1 activity was observed in our system at concentrationsas low as 2 nM, whereas higher doses of bortezomib did not showany effect. This behavior was not related to a toxic effectof bortezomib because we find that this drug did not induceapoptosis or inhibit proliferation of either osteoblast progenitorsor osteoblasts at concentration ranging between 2 and 5 nM.Thus, on the basis of this in vitro evidence, we can supposethat low doses of bortezomib rather than higher ones could bemore effective to stimulate osteoblastogenesis with a relevantclinical perspective in MM patients. A similar behavior on boneformation was previously reported with bisphosphonates thatmay increase osteoblastogenesis in vitro at low doses.²⁵
The stimulatory effect of bortezomib on Runx2/Cbfa1 activityand the related osteoblast markers was further confirmed bythe finding that bortezomib increased bone nodule formationby human PreOBs. A similar effect was observed using specificproteasome inhibitors as MG-132 and MG-262 indicating that thepro-osteogenic effect of bortezomib is due to its capacity toblock proteasome activity in osteoblast and osteoblast progenitors.
In vitro observations were expanded and confirmed in vivo bythe finding of a significant increase of the number of osteoblasticcells and Runx2/Cbfa1-positive cells in MM patients respondingto bortezomib treatment. Based on our evidence, we can supposethat bortezomib may directly stimulate osteoblast differentiation.Alternatively, the rapid apoptosis of MM cells induced by bortezomiband their removal from the BM could result in the recovery ofosteoblast differentiation and an increase in the number ofosteoblastic cells as also demonstrated by the elevation ofbone alkaline phosphatase levels in MM patients responding tobortezomib therapy.^15–17
To have a better overall picture of bone formation and bonedestruction in our group of MM patients, we checked the levelsof serum CTX, a marker of bone resorption that has been demonstrateduseful to evaluate osteoclast activity in MM patients.^26,27In our cohort of MM patients, despite the reduction of serumCTX levels after bortezomib treatment, we failed to find a statisticalsignificance. This observation could be due to either the lownumber of patients in our study or the lower serum CTX levelsat the baseline compared with those reported in another study.²⁸
In conclusion, our data indicate that bortezomib increases osteoblastdifferentiation in human mesenchymal cells without affectingthe number of osteoblast progenitors and the viability of matureosteoblasts. In vivo and in vitro observations support the hypothesisthat both direct and indirect effects on bone formation processcould occur during bortezomib treatment.

   Authorship

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Patients, materials, and methods
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Contribution: N.G. designed the research, analyzed the data,and wrote the paper; F.M. performed all cell culture experimentsand MM cell purification; S.T. performed molecular biology andarray methodologies; M.L. performed immunohistochemistry; S.B.contributed to the characterization of patients; M.C. includedpatients in the study and performed bone biopsies; C.M. contributedto immunohistochemistry and histomorphometry; E.M. contributedto immunohistochemistry and histomorphometry; L.F. contributedto cell culture experiments; A.T. included patients in the study;V.R. provided vital reagents and contributed to the criticalrevision of the paper.
Conflict-of-interest disclosure: The authors declare no competingfinancial interests.
Correspondence: Nicola Giuliani, Hematology and BMT Center,Department of Internal Medicine and Biomedical Science, Universityof Parma, via Gramsci 14, 43100 Parma, Italy; e-mail: nicola.giuliani{at}unipr.it;n_giuliani{at}yahoo.com.

   Acknowledgments

This work was supported by an International Myeloma Foundation(IMF) Grant. We thank the "Associazione Italiana Contro le Leucemie"(AIL) Parma section for the support.
We thank Janssen-Cilag for the financial support for vital reagentsused in the study.
We thank Dr Simona Colla and Dr Marina Magnani for criticalrevision of the paper.

   Footnotes

Submitted November 22, 2006; accepted March 14, 2007.
Prepublished online as Blood First Edition Paper, March 19, 2007 DOI: 10.1182/blood-2006-11-059188

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 USC section 1734.

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