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Prepublished online as a Blood First Edition Paper on August 8, 2002; DOI 10.1182/blood-2002-03-0799.
CLINICAL OBSERVATIONS, INTERVENTIONS, AND THERAPEUTIC TRIALS
From Cellular Transplantation Biology, Kanazawa
University Graduate School of Medical Science; Blood Transfusion
Section, Kanazawa University Hospital, Kanazawa, Ishikawa,
Japan; and the Division of Hematology, Fujigaoka Hospital,
Showa University School of Medicine, Yokohama, Kanagawa,
Japan.
A minor population of blood cells deficient of
glycosylphosphatidylinositol (GPI)-anchored membrane proteins is often
detected in patients with aplastic anemia (AA), though the clinical
significance of such paroxysmal nocturnal hemoglobinuria (PNH)-type
cells remains unclear. To clarify this issue, we studied 164 patients
with myelodysplastic syndrome (MDS) for the presence of
CD55 An increase of blood cells with a paroxysmal
nocturnal hemoglobinuria (PNH) phenotype is often detected in patients
with acquired aplastic anemia (AA).1-6 We previously
demonstrated that a minor (less than 1%) population of
CD55 Myelodysplastic syndrome (MDS) is a clonal disorder of hematopoiesis
characterized by cytopenia and bone marrow dysplasia.8 Because the syndrome is diagnosed on the basis of morphologic abnormalities of blood cells, its pathophysiology is more heterogeneous than that of AA. Among the subtypes of MDS, the diagnosis of refractory anemia (RA) is particularly ambiguous because of the low percentage of
immature blasts.9,10 Some patients with bone marrow
failure may receive diagnoses of RA because of the presence of
slight morphologic abnormalities, despite the fact that their immune pathophysiology is similar to that of typical AA patients. There is no
good marker for distinguishing such a benign subset of RA from other RA
occurrences that are potentially malignant.
Dunn et al11 demonstrated that MDS patients with increases
in the proportion of
CD15+CD16 Therefore, using sensitive flow cytometry that could detect as few as
0.002% PNH-type cells, we examined the peripheral blood of MDS
patients for the presence of PNH-type granulocytes and red blood cells
(RBCs).7 In contrast to previous findings in MDS
patients11 and our own findings in AA
patients,7 increased PNH cells were detected only in a
small subset of RA patients. The PNH+ RA patients showed
benign clinical features distinct from those of PNH Study subjects
Detection of PNH-type cells
PIG-A gene analysis
Typing of HLA-DRB1 alleles HLA-DR serotypes were determined using a lymphocyte toxicity assay (class 2 lambda monoclonal trays; One Lambda, Canoga Park, CA). For patients with DR15, DRB1 alleles were determined by PCR with sequence-specific primers (Dynal classic SSP DRB1*15/16; Dynal, Bromborough Wirral, United Kingdom). For the other patients whose DR serotypes were unknown, only the presence or absence of DRB1*1501 and DRB1*1502 was determined using the same kit.Cyclosporine therapy Cyclosporin A (6 mg/kg per day; Novartis, Basel, Switzerland) was administered to 17 patients after an analysis of PNH-type cells. Responses were evaluated 6 months after therapy. Response criteria included the resolution of a requirement for transfusion and a 2 g/dL or greater increase in hemoglobin level.Statistical analysis Differences of data between PNH+ and PNH patients were assessed using the Fisher exact test
and the Mann-Whitney U test. P < .05 was
considered statistically significant.
Detection of PNH-type granulocytes and RBCs The flow cytometry we used could reliably detect as little as 0.002% CD11b+CD55CD59 cells
within the granulocytes gate, as we previously reported (Figure
1).7 When granulocytes and RBCs were examined, the percentage of PNH-type cells detected was generally different for
granulocytes and RBCs. In patients with low (0.01%) percentages of
PNH-type cells in 2 lineages of cells, PNH-type RBCs were more easily
recognized than PNH-type granulocytes because of a distinct cluster of
glycophorin A+CD55CD59 cells
(Figure 2). Thus, the detection of
PNH-type RBCs in addition to PNH-type granulocytes appeared to
substantiate a diagnosis of bone marrow failure with a minor PNH-type
cell population. Among 68 healthy controls, 26.5% exhibited 1 or 2 CD55CD59 cells per 100 000 granulocytes,
and 50.0% exhibited 1 or 2 CD55CD59 cells
per 100 000 RBCs. However, there was no healthy control who exhibited
3 or more CD55CD59 cells per 100 000
granulocytes and 100 000 RBCs. To avoid false-positive results, the
presence of more than 0.003% CD55CD59
cells in granulocytes and RBCs was arbitrarily defined as an increase
in PNH-type cells.
PIG-A gene abnormalities in a minor population of PNH-type granulocytes A minor population of PNH-type granulocytes was enriched from 5 RA patients by aerolysin treatment, and all exons of the PIG-A gene in these granulocytes were examined using heteroduplex analysis followed by subcloning and sequencing. Table 1 summarizes abnormalities of the PIG-A gene in each patient. Although the proportions of PNH-type cells in these patients were low (0.56 to 2.41%), various abnormalities were detected in all patients.
Prevalence of patients with increased PNH-type blood cells among patients with MDS A significant increase of PNH-type cells was detected in 21 of 119 (17.6%) RA patients. In contrast, increased PNH-type cells were not detected in any of the 4 RARS, 33 RAEB, or 8 RAEB-t patients. Table 2 summarizes the clinical data on the 21 PNH+ RA patients. Bone marrow aspirates from the sternum were hypercellular or normocellular in most patients, though bone marrow biopsy from the iliac bone marrow showed hypocellularity in 10 of 14 patients tested. The percentage of PNH-type granulocytes varied from 0.003% to 2.41% and was less than 1.0% in 17 of 21 (81.0%) PNH+ patients. These low percentages would have been considered insignificant in previous studies. All samples of PNH+ RA patients who exhibited less than 0.01% PNH-type cells were reexamined within 1 month and gave similar results. Nine patients did not require treatment because their pancytopenia remained stable or improved spontaneously. The other 12 patients were treated with cyclosporine or anabolic steroids, and all of them, except patients 3 and 9, improved.
Clinical features of PNH+ RA patients compared with
PNH RA patients to
analyze the clinical significance of the minor population of PNH-type
cells. Table 3 summarizes the results of
the comparison. Thirty-three percent of PNH RA patients
had various karyotypic abnormalities, such as monosomy 7 and trisomy 8, whereas only 1 of 21 PNH+ RA patients had a karyotypic
abnormality of 46,XX,t(6;8)(q15;q22) in 11 of 20 dividing cells. When
the degree of dysplasia was compared using the percentage of
neutrophils with the Pseudo-Pelger-Hüet anomaly in the bone
marrow as a marker, PNH+ RA patients showed significantly
lower percentages of dysplastic neutrophils than PNH RA
patients. The median platelet count (31 × 109/L) in
PNH+ RA patients was significantly lower than that in
PNH RA patients (91 × 109/L;
P = .01).
The most remarkable difference between the 2 groups was the frequency
of HLA-DR15, a split antigen of HLA-DR2. Nineteen of 21 (90.5%)
PNH+ RA patients had HLA-DRB1*1501 or HLA-DRB1*1502,
whereas only 5 of 27 (18.5%) PNH Seventeen RA patients were treated with cyclosporine for more than 3 months after examination of the levels of PNH-type cells. None of the 8 PNH
This study on a large number of MDS patients revealed that increased PNH-type cells were detected in a limited number of patients with RA resembling AA. The flow cytometric assay that we used could reveal the presence of increased PNH-type granulocytes with various PIG-A gene mutations when their percentages were less than 1% of CD11b+ granulocytes. Even with this sensitive flow cytometry, increased PNH-type cells were detected only among RA patients at a much lower prevalence (17.6%) than among the AA patients (52.0%) we reported previously.7 The prevalence of PNH+ patients among all our MDS patients was 12.8%. This lower prevalence, compared with AA patients, was in sharp contrast to the results of a previous report that showed similar prevalence between AA and MDS patients.11,17 This was probably because of the differences in the study population and the specificity of flow cytometric assays used. In contrast to the recent report by Maciejewski et al,17 none of our 68 healthy controls exhibited more than 0.003% PNH-type cells in granulocytes and RBCs. Our failure to detect a single patient with increased PNH-type cells among RARS, RAEB, and RAEB-t patients indicates that the presence of increased PNH-type cells in MDS patients has little to do with the preleukemic nature and that, except for part of RA, MDS is a bone marrow failure distinct from AA in view of the prevalence of PNH-type cells. The absence of karyotypic abnormalities and the progression to advanced MDS or AML in PNH+ RA patients support these hypotheses. In addition to the study by Dunn et al11 that detected more
than 1% CD15+CD16 All the mutations we found in the PNH+ RA patients were in exons 4 and 5. This may be surprising because many of the mutations reported previously were in exons 2 and 6. Iwanaga et al18 demonstrated that 2 of 4 RA patients with increased PNH cells showed a mutation in exon 4 or a deletion of exon 5. It is possible that PIG-A mutations in a minor population of PNH cells from RA patients may be biased toward exons 4 and 5 rather than exons 2 and 6. However, mutations in exons 4 and 5 are not rare, according to a recent paper19 reviewing PIG-A gene analysis on 80 PNH patients. Thus, this possibility must be tested through the study of a larger number of RA patients with increased numbers of PNH- type cells. The most striking feature of our RA patients who had a minor population of PNH-type cells was the high frequency of HLA-DR15. This DR antigen has been repeatedly reported to be associated with susceptibility to AA.20,21 The frequency of HLA-DR15 in PNH+ RA patients (90.5%) in the present study was higher than the frequency of HLA-DR2 (74%) in the recent study by Maciejewski et al.22 This is probably because of the difference in the definition of PNH+ patients. RA patients with a minor population of PNH-type cells may be more likely to have HLA-DR15 than RA patients with 1% or more PNH-type cells. Among DRB1 alleles of HLA-DR15, the presentation of DRB1*1501 by AA patients21,23,24 and MDS patients25 has been linked to a good response to cyclosporine therapy. In keeping with this well-known association, 5 of 5 PNH+ RA patients in the present study who had DRB1*1501 responded to cyclosporine. These findings further support the hypothesis that the minor population of PNH-type cells detected in RA patients reflects the involvement of immune mechanisms in the development of bone marrow failure. One might be concerned about the diagnosis of RA in our
PNH+ patients because the extent of dysplasia in the blood
cells of PNH+ patients was not as severe as that in
PNH The results of the present study may have important implications for clinical practice. Although several studies have shown that considerable proportions of MDS patients experience restoration of hematopoietic function with immunosuppressive therapy,31-34 there has been no marker for a good response to the therapy. The presence of a minor population of PNH+ cells may serve as such a marker for immune-mediated bone marrow failure. PNH+ RA patients have probably been overlooked because of difficulties in detecting a minor population of PNH-type cells with conventional flow cytometry. They may have been treated with toxic therapy, such as bone marrow transplantation from unrelated donors and low-dose cytosine arabinoside. A prospective study in a larger group of patients is needed to establish the clinical significance of PNH-type cells in the management of bone marrow failure.
We thank the following physicians for providing us with patient samples and clinical information: K. Ohyashiki, Tokyo Medical University; H. Yamauchi, Kurobe City Hospital; H. Yamazaki, Toyama City Hospital; K. Kyoda, Fukuiken Saiseikai Hospital; K. Masuda, Okayama University Hospital; M. Saito, NTT Kanazawa Hospital; M. Teramura, Tokyo Women's Medical College; M. Ueda, Ishikawa Prefectural Central Hospital; N. Ichikawa, Nagano Red Cross Hospital; S. Fujii, Teraoka Memorial Hospital; S. Matano, Tonami General Hospital; T. Nakamoto, Tokyo University Hospital; and T. Yoshida, Toyama Prefectural Central Hospital.
Submitted March 18, 2002; accepted July 15, 2002.
Prepublished online as Blood First Edition Paper, August 8, 2002; DOI 10.1182/blood-2002-03-0799.
Supported in part by a Grant-in-Aid for Immunologic Research for Intractable Diseases from the Ministry of Health, Labor and Welfare of Japan.
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: Shinji Nakao, Cellular Transplantation Biology, Kanazawa University Graduate School of Medical Science, 13-1 Takaramachi, Kanazawa, Ishikawa, Japan 920-8641; e-mail: snakao{at}med3.m.kanazawa-u.ac.jp.
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  R. A. Brodsky Narrative Review: Paroxysmal Nocturnal Hemoglobinuria: The Physiology of Complement-Related Hemolytic Anemia Ann Intern Med, April 15, 2008; 148(8): 587 - 595. [Full Text] [PDF]
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 H. Takamatsu, X. Feng, T. Chuhjo, X. Lu, C. Sugimori, K. Okawa, M. Yamamoto, S. Iseki, and S. Nakao Specific antibodies to moesin, a membrane-cytoskeleton linker protein, are frequently detected in patients with acquired aplastic anemia Blood, March 15, 2007; 109(6): 2514 - 2520. [Abstract] [Full Text] [PDF]
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C. Sugimori, T. Chuhjo, X. Feng, H. Yamazaki, A. Takami, M. Teramura, H. Mizoguchi, M. Omine, and S. Nakao Minor population of CD55-CD59- blood cells predicts response to immunosuppressive therapy and prognosis in patients with aplastic anemia Blood, February 15, 2006; 107(4): 1308 - 1314. [Abstract] [Full Text] [PDF]
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 R. A. Brodsky New Insights into Paroxysmal Nocturnal Hemoglobinuria Hematology, January 1, 2006; 2006(1): 24 - 28. [Abstract] [Full Text] [PDF]
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J. W. Vardiman Hematopathological Concepts and Controversies in the Diagnosis and Classification of Myelodysplastic Syndromes Hematology, January 1, 2006; 2006(1): 199 - 204. [Abstract] [Full Text] [PDF]
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Top
Abstract
Introduction
