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BRIEF REPORT
From the Departments of Pediatrics and Transfusion
Medicine, University of Ulm, Ulm, Germany.
Infantile osteopetrosis (OP) carries an extremely poor
prognosis unless treated early by hematopoietic stem cell
transplantation. We explored the use of purified blood progenitor cells
from HLA-haploidentical parents in 7 patients lacking suitable matched
donors. Blood progenitor cells were purified by positive selection and
by additional T-cell depletion using rosette formation. For
conditioning, patients received busulfan, thiotepa, and either
cyclophosphamide (5 patients) or fludarabine (2 patients). Stable donor
engraftment developed in 6 of 7 patients. Graft-versus-host disease was
not observed. Three of the 7 patients had no major complications and 4 of 7 had both veno-occlusive disease and respiratory failure. Five of 7 patients survive with complete cure of OP at a median of 4 years.
Patients with OP lacking HLA-matched donors can be successfully treated
by transplantation of purified blood progenitor cells from
HLA-haploidentical donors.
(Blood. 2002;99:3458-3460) Osteopetrosis (OP) represents a group of disorders
characterized by excessive bone density due to defective osteoclast
function.1 Recently in patients with the severe autosomal
recessive variant of the disorder (malignant infantile OP) mutations
were described in genes expressed in osteoclasts affecting ion channel
proteins.2-4 One gene, encoding the a3 subunit of the
vacuolar H+-ATPase, was found to be affected in 10 of 19 patients with OP, including 5 of the 7 patients presented in this
paper (2 patients were not analyzed). Osteoclasts are of hematopoietic
origin, and hematopoietic stem cell transplantation (HSCT) represents
an effective treatment.1,5 Because of the usually rapid
development of complications such as hematologic failure and
irreversible sensoneurologic impairment, treatment needs to be
initiated expeditiously. The lack of a suitable, HLA-compatible donor
and the low success rate using alternative donors have limited this
strategy so far.6
In the HLA-nonidentical setting, the use of T cell-depleted
transplants prevents complications of graft-versus-host disease (GVHD).
This approach has been successful in particular in children with
primary immunodefiencies,7-9 whereas in patients with
other congenital disorders including OP it has been complicated so far by high graft failure rates.10,11 Recently results of
HLA-nonidentical HSCT improved markedly using large numbers of
granulocyte colony-stimulating factor (G-CSF)-mobilized, T
cell-depleted peripheral blood progenitor cells.12-14 In
the current study, we explored the use of purified blood progenitor
cells from HLA-haploidentical parents in the treatment of 7 infants
with malignant OP.
Patients
Transplantation procedure
Stem cell preparation To mobilize CD34+ progenitor cells, donors were treated with recombinant human G-CSF (rHuG-CSF; Lenograstim, Rhône-Poulenc, Cologne, Germany) at 10 µg/kg per day subcutaneously for 4 to 5 days. Donor leukocytes were obtained by apheresis using a COBE Spectra Cell Separator (COBE BCT, Heimstetten, Germany). CD34+ cells were isolated by positive selection using in 4 initial cases the CeprateSC device (Cellpro, Brussels, Belgium) and in 2 others by the CliniMACS system (Miltenyi Biotec, Bergisch Gladbach, Germany).15 Residual T cells were further depleted by rosetting with human erythrocytes coated with anti-CD3+ and anti-CD2+ as described elsewhere.14 Numbers of CD34+ cells and CD3+ cells in the grafts were determined by flow cytometry. Transplanted stem cell numbers ranged from 12 to 56 × 106/kg (median 30 × 106/kg) and transplanted T-cell numbers from 0.8 to 11.1 × 104/kg (median 1.7 × 104/kg). All patients except one received additional infusions of cryopreserved donor CD34+ cells as a boost. These cells were given early (between day 7 and 11) in 5 cases and late (day 42) in 2 cases, ranging in numbers from 10 × 106/kg to 43 × 106/kg (median 15 × 106/kg; Table 2). Recipients received rHuG-CSF until stable engraftment was achieved. Besides T-cell depletion, no further GVHD prophylaxis was administered.Analysis of engraftment Engraftment of donor cells was analyzed by repeated HLA-typing of peripheral blood leukocytes and by blood group determination. Immunologic reconstitution was evaluated by monitoring the number of circulating T cells and B cells and by repeated determination of T- and B-cell functions as described.14
Transplant courses were accompanied by a high rate of toxic and infectious complications (Table 2). Thus, severe respiratory problems requiring mechanical ventilation developed in 4 cases: UPN 275 and UPN 292 because of cytomegalovirus (CMV) pneumonitis, UPN 303 due to respiratory failure from severe airway obstruction, and UPN 323 due to late veno-occlusive disease (VOD) of the lung. Each of these 4 patients also developed hepatic VOD, representing an unusually high incidence of this complication. The use of intensive conditioning, the young age of our patients at transplantation as well as disease-specific problems related to the underlying disorder may account for this increased risk to develop transplant-related complications. In an attempt to lower this risk, in particular of VOD, an alternative conditioning was evaluated in 2 more recent cases, replacing 1 of the 2 alkylating agents, namely cyclophosphamide, by fludarabine. This regimen led to markedly reduced toxicity with absence of VOD, and although limited, warrants further exploration in additional patients. In 5 of the 7 cases sustained engraftment of donor cells was observed. Two patients developed graft failures: in patient UPN 275 graft function deteriorated at 1 month in the context of CMV disease, which was reversible by a second graft on day 42 from the same donor without further conditioning. This complication may reflect the vulnerability of the reconstituting hematopoietic system after purified blood progenitor cell transplantation. In the other patient (UPN 292) the graft was rejected on day +15, following conditioning with a lowered total dose of cyclophosphamide (120 mg/kg instead of 200 mg/kg). This child died from CMV pneumonia shortly after a second transplant from the opposite parent. Graft rejection in this case may emphasize the critical role of the intensity of conditioning, even if high numbers of stem cells are used for transplantation. It should also be pointed out that in the other patients complete hematologic recovery with development of normal blood cell counts was delayed (Table 2). This delay may be related to the occlusion of marrow space characteristic for the disease. In an attempt to shorten the time interval to hematologic recovery, additional donor CD34+ cells were infused at around 1 week after HSCT in 5 of the 7 patients. Although no effect on the slow kinetics of hematologic recovery was evident, regardless of the number of CD34+ cells infused, this approach may have led to stabilization of engraftment, because none of the patients developed graft failures. Two patients received late boosts of CD34+ cells at day 42 because of persistent marked tricytopenia in one (UPN 332) and because of secondary graft failure in the other (UPN 275 mentioned above). In both patients rapid normalization of blood cell counts was observed, suggesting that delayed boosts may improve hematopoietic functions after HSCT in OP. T-cell immunity by donor cells developed with a delay of 3 to 6 months, regardless of the total number of CD34+ cells infused (data not shown). No patient developed acute or chronic GVHD. Five of 7 patients survive for 25 to 60 months (median, 47 months). In these patients, the disease regressed as demonstrated by normalization of hematopoietic function, regular calcium homeostasis, and reversal of hepatosplenomegaly. One patient (UPN 303) developed portal vein thrombosis, possibly as a late complication of hepatic VOD and also shows developmental retardation of unknown origin at 4 years after transplantation. Visual impairment due to optical nerve atrophy present at the time of transplantation in 4 of the surviving patients remained unchanged. Other serious neurologic sequelae are absent. As demonstrated by repeat bone marrow biopsies and by serial skeletal radiograms, structural abnormalities of the skeletal system improved gradually, normalizing at around 1 year after transplantation. Repeat chimerism analysis revealed stable donor cell engraftment in all surviving patients. The outcome of HLA-haplotype mismatched SCT for treatment of OP has been disappointingly poor so far, with survival rates of only 10% (data of the European Bone Marrow Transplantation study, the International Bone Marrow Transplant Registry and the National Marrow Donor Program, reviewed by Fasth and Porras6 and Gerritsen et al16). In this study we explored a novel approach using high numbers of purified CD34+ blood progenitor cells from related family donors. In addition we applied an intensive triple-drug conditioning regimen incorporating also anti-T-cell antibodies for additional immunosuppression. It is not possible to dissect the respective roles of the hematopoietic grafts and the intensive immunosuppression used for the observed low rate of graft failure and the improved survival rate. Nevertheless, our finding of stable donor cell engraftment in 6 of 7 cases and of cure of disease in 5 of 7 patients is encouraging. Because of the usually rapid progression of the disease, HSCT needs to be performed as early as possible after diagnosis, and the approach used in our study makes this feasible.
Submitted August 21, 2001; accepted December 4, 2001.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Ansgar S. Schulz, Department of Pediatrics, University of Ulm, Prittwitzstr. 43, D-89075 Ulm, Germany; e-mail: ansgar.schulz{at}gmx.de.
1.
Felix R, Hofstetter W, Cecchini MG.
Recent developments in the understanding of the pathophysiology of osteopetrosis.
Eur J Endocrinol.
1996;134:143-156 2. Frattini A, Orchard PJ, Sobacchi C, et al. Defects in TCIRG1 subunit of the vacuolar proton pump are responsible for a subset of human autosomal recessive osteopetrosis. Nat Genet. 2000;25:343-346[CrossRef][Medline] [Order article via Infotrieve].
3.
Kornak U, Schulz A, Friedrich W, et al.
Mutations in the a3 subunit of the vacuolar H+-ATPase cause infantile malignant osteopetrosis.
Hum Mol Genet.
2000;9:2059-2063 4. Kornak U, Kasper D, Bösl MR, et al. Loss of the CIC-7 chloride channel leads to osteopetrosis in mice and man. Cell. 2001;104:205-215[CrossRef][Medline] [Order article via Infotrieve]. 5. Coccia PF, Krivit W, Cervenka J, et al. Successful bone-marrow transplantation for infantile malignant osteopetrosis. N Engl J Med. 1980;302:701-708[Abstract]. 6. Fasth A, Porras O. Human malignant osteopetrosis: pathophysiology, management and the role of bone marrow transplantation. Pediatr Transplant. 1999;3(suppl):102-107.
7.
Reisner Y, Kapoor N, Kirkpatrick D, et al.
Transplantation for severe combined immunodefiency with HLA-A, B, D, DR incompatible parental marrow cells fractionated by soybean agglutination and sheep red blood cells.
Blood.
1983;61:341-348 8. Friedrich W, Goldmann S, Ebell W, et al. Severe combined immunodeficiency: treatment by bone marrow transplantation in 15 infants using HLA-haploidentical donors. Eur J Pediatr. 1985;144:125-130[CrossRef][Medline] [Order article via Infotrieve]. 9. Fischer A, Landais P, Friedrich W, et al. European experience of bone marrow transplantation for severe combined immunodefiency. Lancet. 1990;226:850-854. 10. O'Reilly RJ, Collins N, Kernan NA, et al. Transplantation of marrow depleted of T cells by soybean lectin agglutination and E-rosette depletion: major histocompatibility complex-related graft resistance in leukemic transplant recipients. Transplant Proc. 1985;17:455-459. 11. Anasetti C, Amos D, Beatty PG, et al. Effect of HLA compatibility on engraftment of bone marrow transplants in patients with leukemia or lymphoma. N Engl J Med. 1989;17:197-204.
12.
Aversa F, Tabilio A, Velardi A, et al.
Treatment of high-risk acute leukemia with T-cell-depleted stem cells from related donors with one fully mismatched HLA haplotype.
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1998;339:1186-1193
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Aversa F, Terenzi A, Carotti A, et al.
Improved outcome with T-cell-depleted bone marrow transplantation for acute leukemia.
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1999;17:1545-1550 14. Mueller S, Schulz A, Reiss U, et al. Definition of a critical T cell threshold for prevention of GVHD after HLA non-identical PBPC transplantation in children. Bone Marrow Transplant. 1999;24:575-581[CrossRef][Medline] [Order article via Infotrieve]. 15. Wiesneth M, Schreiner T, Friedrich W, et al. Combined CD34 positive plus CD2 negative selection for effective T-cell depletion as GvHD prophylaxis in HLA-nonidentical blood progenitor cell transplantation. Transfus Sci. 1996;17:629-635[Medline] [Order article via Infotrieve]. 16. Gerritsen EJ, Vossen JM, Fasth A, et al. Bone marrow transplantation for autosomal recessive osteopetrosis. A report from the Working Party on Inborn Errors of the European Bone Marrow Transplantation Group. J Pediatr. 1994;125:896-902[CrossRef][Medline] [Order article via Infotrieve].
© 2002 by The American Society of Hematology.
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  A. Frattini, H. C. Blair, M. G. Sacco, F. Cerisoli, F. Faggioli, E. M. Cato, A. Pangrazio, A. Musio, F. Rucci, C. Sobacchi, et al. Rescue of ATPa3-deficient murine malignant osteopetrosis by hematopoietic stem cell transplantation in utero PNAS, October 11, 2005; 102(41): 14629 - 14634. [Abstract] [Full Text] [PDF]
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Abstract
Introduction