Blood Res 2014; 49(1):
Published online March 31, 2014
https://doi.org/10.5045/br.2014.49.1.22
© The Korean Society of Hematology
1Department of Laboratory Medicine, Catholic Blood and Marrow Transplantation Center, The Catholic University of Korea, Seoul, Korea.
2Department of Hematology, Department of Internal Medicine, Catholic Blood and Marrow Transplantation Center, The Catholic University of Korea, Seoul, Korea.
Correspondence to : Correspondence to Myungshin Kim, M.D., Ph.D. Department of Laboratory Medicine, Seoul St. Mary's Hospital, College of Medicine, The Catholic University of Korea, 222 Banpo-daero, Seocho-gu, Seoul 137-701, Korea. Tel: +82-2-2258-1645, Fax: +82-2-2258-1719, microkim@catholic.ac.kr
This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
The coexistence of t(9;22)(q34;q11.2) and inv(16)(p13q22) chromosomal abnormalities is extremely uncommon, and only a small number of such cases have been reported. Here, we characterized 7 cases of hematologic malignancy exhibiting t(9;22) and inv(16) coexistence.
We reviewed the cytogenetic data for hematologic malignancies treated at the Catholic Blood and Marrow Transplantation Center between January 2004 and June 2013. We identified 7 cases exhibiting t(9;22) and inv(16) coexistence. In addition, we analyzed mutations in the
Four cases of chronic myelogenous leukemia (CML; 1 chronic phase, 2 accelerated phase, and 1 blast phase) and 3 cases of acute myeloid leukemia (AML; 1 de novo and 2 therapy-related) were identified. The percentages of circulating blasts and bone marrow eosinophils were higher in AML cases than in CML cases (53% vs. 5% and 30% vs. 5.5%, respectively). The proportions of each chromosomal abnormality were used along with follow-up karyotyping results to identify secondary changes. In
This study shows that observations of bone marrow morphology, initial and follow-up cytogenetic studies, and karyotyping of
Keywords Chronic myelogenous leukemia, Acute myeloid leukemia, t(9;22),
The presence of chromosomal abnormalities, including inv(16)(p13q22) and its associated variant-t(16;16)(p13;q22), in acute myeloid leukemia (AML) is relatively common. Such abnormalities occur in 10%-12% of all AML cases [1]. AML with inv(16) has been defined as a distinctive morphologic subtype and is designated M4Eo by the French-American-British Cooperative Group. From a molecular standpoint, the inversion of chromosome 16 creates the pathologic fusion gene
We reviewed all cytogenetic data for patients with hematologic malignancies who received treatment at the Catholic Blood and Marrow Transplantation Center between January 2004 and June 2013. We observed 716 cases of t(9;22), including 705 with CML, 151 cases of acute lymphoblastic leukemia/acute biphenotypic leukemia, and 56 cases of AML. AML with inv(16) occurred in 104 cases. Among these cases, we identified 7 patients exhibiting both t(9;22) and inv(16). This study was performed according to the Declaration of Helsinki guidelines, and full approval was obtained from the institutional review board of St. Mary's Hospital, which is affiliated with The Catholic University of Korea (IRB No: KC13ZISE0779).
We reviewed all available data, including peripheral blood (PB) smears, bone marrow (BM) aspirates, cytochemical staining, and core biopsy specimens. Clinical information was also reviewed when available; however, not all cases included the same types of data. Immunophenotyping of cells was performed with flow cytometry against CD3, CD41a, CD14, CD34, CD33, CD20, CD5, CD10, CD19, CD64, CD11c, CD13, CD117, CD56, CD2, CD7, HLA-DR, cytoplasmic CD22, cytoplasmic myeloperoxidase, cytoplasmic CD3, and cytoplasmic CD79a (BD Biosciences, San Jose, CA, USA). Leukemic blasts were analyzed with the FACSDiva program (BD Biosciences).
Chromosomal analyses were performed by examining short-term cultures of BM specimens according to standard conventional cytogenetic protocols. At least 20 cells in metaphase were analyzed in each case. Clonal abnormalities were classified according to the 2009 International System for Human Cytogenetic Nomenclature guidelines [7].
In 6 of 7 cases, fluorescence in situ hybridization (FISH) analyses were performed to confirm Ph translocation and the presence of inv(16). These FISH analyses used pellets of cells remaining after conventional cytogenetic studies. Slides for FISH were prepared by using cells harvested for conventional cytogenetics and processing them for FISH according to the manufacturer's guidelines (Abbott Vysis, Des Plaines, IL, USA). Analyses were performed on cells in either interphase or metaphase. An LSI
RNA from 6 patients was extracted from BM cells, reverse transcribed into complementary DNA using a QIAamp RNA Blood Mini Kit (Qiagen, Chatsworth, CA, USA) according to the manufacturer's instructions, and analyzed using RT-PCR designed to detect the
Genomic DNA was extracted from BM specimens using a QIAamp DNA Blood Mini Kit (Qiagen, Hilden, Germany). We analyzed an internal tandem duplication in
The clinical and laboratory characteristics of the patients analyzed in this study are summarized in Table 1. In total, 5 men and 2 women with a median age of 27 years (range, 10-61 years) were included. Four cases of CML and 3 cases of AML were identified. The incidence of inv(16) in the patients with CML was 0.6% (4/705), and the incidence of t(9;22) in patients with AML with inv(16) was 2.9% (3/104). Among the 4 CML patients, 1 patient (case 2) presented with CML-chronic phase (CML-CP). Two patients were previously diagnosed with and treated for CML-CP and later progressed to CML-BP (cases 1 and 4). One patient initially presented with CML-BP. Among the 3 patients diagnosed with AML, 1 had de novo AML M4Eo and the other 2 were diagnosed with t-AML. One t-AML patient presented with Hodgkin's lymphoma and was treated with doxorubicin, bleomycin, vinblastine, and dacarbazine chemotherapy (case 6), and the other presented with follicular lymphoma and was treated with fludarabine, mitoxantrone, and dexamethasone chemotherapy (case 7). Splenomegaly was documented in all cases except case 3. All patients received chemotherapy containing imatinib mesylate (Table 2). Two patients with CML and 3 patients with AML underwent either BM or PB stem cell transplantation. One patient died of sepsis 5 months after developing CML-BP (case 3). The other 6 patients were alive at the most recent follow-up examination.
In the CML cases, clinical studies of PB revealed anemia (median Hb, 9.1 g/dL) and mild to severe leukocytosis (median WBC, 134.1×109/L). Thrombocytosis was observed in 2 patients with CML (cases 2 and 3). The other 2 patients with CML exhibited thrombocytopenia. In the AML cases, clinical studies of the PB revealed anemia (median Hb, 8.3 g/dL) and mild leukocytosis (median WBC, 91.3×109/L). All AML patients also exhibited thrombocytopenia (median platelet count, 29×109/L). The percentage of circulating blasts was variable and higher in AML patients than in CML patients (median, 53% vs. 5%,
The cytogenetic and molecular findings of this study are summarized in Table 2. All patients exhibited t(9;22) and inv(16) at some point during the course of their disease. Five patients showed complex karyotypes with additional numerical chromosomal aberrations, structural chromosomal aberrations, or both. Of the 4 patients with CML, 1 patient had both abnormalities detected in the CML-CP sample, whereas the other 3 had both abnormalities detected in CML-BP samples. Of the 3 CML-BP cases, 2 cases included karyotype results for the time at which the patients exhibited CML-CP, and both showed t(9;22) without inv(16). Of the 3 patients with AML, 1 of the patients with t-AML (case 7) had the karyotype result from the previous illness, which showed inv(16) without t(9;22). Follow-up karyotype results were available for all patients. Cells in metaphase were documented for all CML-BP cases, with the occurrence of t(9;22) observed only after treatment. One CML-CP and 3 AML cases showed normal karyotype results after treatment.
The
Coexistence of t(9;22) and inv(16) is rare in hematologic malignancies. The few cases in which both of these aberrations have been reported have had either an AML or a CML phenotype (Table 3). In this study, we identified 4 cases of CML and 3 cases of AML, in which both of these chromosomal abnormalities occurred. Although the prevalence of t(9;22) and inv(16) coexistence has not yet been fully evaluated, a previous study showed that the incidence of t(9;22) in AML with inv(16) is less than 1% (approximately 0.5%) [19]. Our data showed that the coexistence of these abnormalities was detected in 0.6% of CML cases and 2.9% of AML cases with inv(16).
The majority of documented AML patients with t(9;22) and inv(16) coexistence have exhibited M4Eo BM morphology, including an increased number of myelomonocytic cells and abnormal eosinophils with coarse basophilic granules [8]. The AML cases we studied had similar AML-M4Eo BM morphologies. However, because the CML-BP cases in this study also exhibited an increased number of myelomonocytic cells and abnormal eosinophils, we had difficulty in discriminating CML-BP from AML on a morphological basis alone. Patients with a history of CML-CP before the development of a "double positive" can be easily diagnosed with CML-BP. However, we found that patients with AML exhibited a higher number of circulating blasts and more severe BM eosinophilia than did patients with CML-BP.
Cytogenetically, the proportion of each chromosomal abnormality was informative for identifying secondary changes [3]. This study documented a CML patient with secondary inv(16) who also exhibited a minor proportion of a
In most double-positive cases, the major p210 chimeric BCR-ABL1 protein is observed in CML, whereas the minor p190 form correlates with AML presentation. However, some exceptions to this tendency have also been reported [9, 21, 22]. In the present study, a p210 fusion was detected in all patients with CML and 1 patient with de novo AML; moreover, a p190 fusion was detected in the 2 patients with t-AML. These findings suggest that the presence of a p190 BCR-ABL1 fusion protein is associated with AML. In addition, rare
We also analyzed the presence of commonly observed mutations associated with inv(16) and t(9;22). Nacheva et al. [24] have shown that AML with t(9;22) is accompanied by the loss of
De novo AML with coexisting t(9;22) and inv(16) chromosomal abnormalities appears to have a prognosis as favorable as that in AML with inv(16) alone, whereas CML with both t(9;22) and inv(16) seems to have an unfavorable or uncertain prognosis [4, 5]. However, our data show that only 1 patient with CML-BP died of sepsis, and the other patients sustained clinical remission. Imatinib mesylate has been used effectively and safely to treat CML-BP [27]. With the benefits of better tolerance and fewer side effects, it has also been useful as a first-line interim therapy or maintenance strategy to bridge hematopoietic stem cell transplantation in patients with AML [28].
An interesting finding in the present study is that the 2 patients with t-AML exhibited t(9;22) and inv(16) coexistence. Patients with t(9;22) represent 2% of all therapy-related cases of myelodysplastic syndromes and t-AML. Moreover, t(9;22) is significantly associated with previous therapy with topoisomerase II inhibitors [5]. Although inv(16) is a well-known recurrent abnormality in t-AML, it is most frequently observed in patients with breast cancer or lymphoma who have been treated with alkylating agents, topoisomerase II inhibitors, radiation therapy, or a combination thereof. The response rates to intensive antileukemic chemotherapy in patients with t-AML with inv(16) are comparable to those of patients with de novo AML. Overall, 85% of all patients obtain complete remission after intensive chemotherapy [29]. In the present study, 1 patient had follicular lymphoma treated with an alkylating agent, and t-AML occurred 14 months after finishing lymphoma treatment. The other t-AML patient had received chemotherapy including topoisomerase II inhibitors for follicular lymphoma and developed t-AML 10 months after completing treatment. Complex karyotype, reportedly the strongest prognostic indicator, predicts a poor prognosis for t-AML patients. One study has reported that the t-AML M3 phenotype has a good prognosis, but overall survival is significantly shorter in t-AML with a complex karyotype [30].
The present study shows that evaluations of the percentage of circulating blasts and BM eosinophils, careful comparison of initial and follow-up cytogenetics studies including FISH results, and karyotyping of
Table 1 Patient characteristics.
a)Phase in which cytogenetic studies were performed.
Abbreviations: AML, acute myeloid leukemia; AP, accelerated phase; Bø, basophil; BP, blast phase; CML, chronic myelogenous leukemia; CP, chronic phase; Eø, eosinophil; Hb, hemoglobin; M4Eo, French-American-British Cooperative Group classification M4 with eosinophils; Nø, neutrophil; Plt, platelet; t-AML, therapy-related AML.
Table 2 Molecular and cytogenetic findings and clinical outcomes.
a)Months from previous diagnosis. b)Months from presence of inv(16) and t(9;22).
Abbreviations: alloPBSCT, allogeneic peripheral blood stem cell transplant; BM, bone marrow; FISH, fluorescence in situ hybridization; ND, not done; RT-PCR, reverse transcriptase-polymerase chain reaction; uBMT, unrelated BM transplantation; uPBSCT, unrelated peripheral blood stem cell transplant.
Table 3 Previously reported cases of t(9;22) and inv(16) coexistence.
Abbreviations: AML, acute myeloid leukemia; AML M1, acute myeloblastic leukemia; allo-BMT, allogeneic bone marrow transplant; BP, blast phase; F, female; M, male; m-bcr, minor breakpoint region; M-bcr, major breakpoint region; M4Eo, French-American-British Cooperative Group classification M4 with eosinophils; ND, not done.
Blood Res 2014; 49(1): 22-28
Published online March 31, 2014 https://doi.org/10.5045/br.2014.49.1.22
Copyright © The Korean Society of Hematology.
Eunhee Han1, Hyeyoung Lee1, Myungshin Kim1*, Yonggoo Kim1, Kyungja Han1, Sung-Eun Lee2, Hee-Je Kim2, and Dong-Wook Kim2
1Department of Laboratory Medicine, Catholic Blood and Marrow Transplantation Center, The Catholic University of Korea, Seoul, Korea.
2Department of Hematology, Department of Internal Medicine, Catholic Blood and Marrow Transplantation Center, The Catholic University of Korea, Seoul, Korea.
Correspondence to: Correspondence to Myungshin Kim, M.D., Ph.D. Department of Laboratory Medicine, Seoul St. Mary's Hospital, College of Medicine, The Catholic University of Korea, 222 Banpo-daero, Seocho-gu, Seoul 137-701, Korea. Tel: +82-2-2258-1645, Fax: +82-2-2258-1719, microkim@catholic.ac.kr
This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.
The coexistence of t(9;22)(q34;q11.2) and inv(16)(p13q22) chromosomal abnormalities is extremely uncommon, and only a small number of such cases have been reported. Here, we characterized 7 cases of hematologic malignancy exhibiting t(9;22) and inv(16) coexistence.
We reviewed the cytogenetic data for hematologic malignancies treated at the Catholic Blood and Marrow Transplantation Center between January 2004 and June 2013. We identified 7 cases exhibiting t(9;22) and inv(16) coexistence. In addition, we analyzed mutations in the
Four cases of chronic myelogenous leukemia (CML; 1 chronic phase, 2 accelerated phase, and 1 blast phase) and 3 cases of acute myeloid leukemia (AML; 1 de novo and 2 therapy-related) were identified. The percentages of circulating blasts and bone marrow eosinophils were higher in AML cases than in CML cases (53% vs. 5% and 30% vs. 5.5%, respectively). The proportions of each chromosomal abnormality were used along with follow-up karyotyping results to identify secondary changes. In
This study shows that observations of bone marrow morphology, initial and follow-up cytogenetic studies, and karyotyping of
Keywords: Chronic myelogenous leukemia, Acute myeloid leukemia, t(9,22),
The presence of chromosomal abnormalities, including inv(16)(p13q22) and its associated variant-t(16;16)(p13;q22), in acute myeloid leukemia (AML) is relatively common. Such abnormalities occur in 10%-12% of all AML cases [1]. AML with inv(16) has been defined as a distinctive morphologic subtype and is designated M4Eo by the French-American-British Cooperative Group. From a molecular standpoint, the inversion of chromosome 16 creates the pathologic fusion gene
We reviewed all cytogenetic data for patients with hematologic malignancies who received treatment at the Catholic Blood and Marrow Transplantation Center between January 2004 and June 2013. We observed 716 cases of t(9;22), including 705 with CML, 151 cases of acute lymphoblastic leukemia/acute biphenotypic leukemia, and 56 cases of AML. AML with inv(16) occurred in 104 cases. Among these cases, we identified 7 patients exhibiting both t(9;22) and inv(16). This study was performed according to the Declaration of Helsinki guidelines, and full approval was obtained from the institutional review board of St. Mary's Hospital, which is affiliated with The Catholic University of Korea (IRB No: KC13ZISE0779).
We reviewed all available data, including peripheral blood (PB) smears, bone marrow (BM) aspirates, cytochemical staining, and core biopsy specimens. Clinical information was also reviewed when available; however, not all cases included the same types of data. Immunophenotyping of cells was performed with flow cytometry against CD3, CD41a, CD14, CD34, CD33, CD20, CD5, CD10, CD19, CD64, CD11c, CD13, CD117, CD56, CD2, CD7, HLA-DR, cytoplasmic CD22, cytoplasmic myeloperoxidase, cytoplasmic CD3, and cytoplasmic CD79a (BD Biosciences, San Jose, CA, USA). Leukemic blasts were analyzed with the FACSDiva program (BD Biosciences).
Chromosomal analyses were performed by examining short-term cultures of BM specimens according to standard conventional cytogenetic protocols. At least 20 cells in metaphase were analyzed in each case. Clonal abnormalities were classified according to the 2009 International System for Human Cytogenetic Nomenclature guidelines [7].
In 6 of 7 cases, fluorescence in situ hybridization (FISH) analyses were performed to confirm Ph translocation and the presence of inv(16). These FISH analyses used pellets of cells remaining after conventional cytogenetic studies. Slides for FISH were prepared by using cells harvested for conventional cytogenetics and processing them for FISH according to the manufacturer's guidelines (Abbott Vysis, Des Plaines, IL, USA). Analyses were performed on cells in either interphase or metaphase. An LSI
RNA from 6 patients was extracted from BM cells, reverse transcribed into complementary DNA using a QIAamp RNA Blood Mini Kit (Qiagen, Chatsworth, CA, USA) according to the manufacturer's instructions, and analyzed using RT-PCR designed to detect the
Genomic DNA was extracted from BM specimens using a QIAamp DNA Blood Mini Kit (Qiagen, Hilden, Germany). We analyzed an internal tandem duplication in
The clinical and laboratory characteristics of the patients analyzed in this study are summarized in Table 1. In total, 5 men and 2 women with a median age of 27 years (range, 10-61 years) were included. Four cases of CML and 3 cases of AML were identified. The incidence of inv(16) in the patients with CML was 0.6% (4/705), and the incidence of t(9;22) in patients with AML with inv(16) was 2.9% (3/104). Among the 4 CML patients, 1 patient (case 2) presented with CML-chronic phase (CML-CP). Two patients were previously diagnosed with and treated for CML-CP and later progressed to CML-BP (cases 1 and 4). One patient initially presented with CML-BP. Among the 3 patients diagnosed with AML, 1 had de novo AML M4Eo and the other 2 were diagnosed with t-AML. One t-AML patient presented with Hodgkin's lymphoma and was treated with doxorubicin, bleomycin, vinblastine, and dacarbazine chemotherapy (case 6), and the other presented with follicular lymphoma and was treated with fludarabine, mitoxantrone, and dexamethasone chemotherapy (case 7). Splenomegaly was documented in all cases except case 3. All patients received chemotherapy containing imatinib mesylate (Table 2). Two patients with CML and 3 patients with AML underwent either BM or PB stem cell transplantation. One patient died of sepsis 5 months after developing CML-BP (case 3). The other 6 patients were alive at the most recent follow-up examination.
In the CML cases, clinical studies of PB revealed anemia (median Hb, 9.1 g/dL) and mild to severe leukocytosis (median WBC, 134.1×109/L). Thrombocytosis was observed in 2 patients with CML (cases 2 and 3). The other 2 patients with CML exhibited thrombocytopenia. In the AML cases, clinical studies of the PB revealed anemia (median Hb, 8.3 g/dL) and mild leukocytosis (median WBC, 91.3×109/L). All AML patients also exhibited thrombocytopenia (median platelet count, 29×109/L). The percentage of circulating blasts was variable and higher in AML patients than in CML patients (median, 53% vs. 5%,
The cytogenetic and molecular findings of this study are summarized in Table 2. All patients exhibited t(9;22) and inv(16) at some point during the course of their disease. Five patients showed complex karyotypes with additional numerical chromosomal aberrations, structural chromosomal aberrations, or both. Of the 4 patients with CML, 1 patient had both abnormalities detected in the CML-CP sample, whereas the other 3 had both abnormalities detected in CML-BP samples. Of the 3 CML-BP cases, 2 cases included karyotype results for the time at which the patients exhibited CML-CP, and both showed t(9;22) without inv(16). Of the 3 patients with AML, 1 of the patients with t-AML (case 7) had the karyotype result from the previous illness, which showed inv(16) without t(9;22). Follow-up karyotype results were available for all patients. Cells in metaphase were documented for all CML-BP cases, with the occurrence of t(9;22) observed only after treatment. One CML-CP and 3 AML cases showed normal karyotype results after treatment.
The
Coexistence of t(9;22) and inv(16) is rare in hematologic malignancies. The few cases in which both of these aberrations have been reported have had either an AML or a CML phenotype (Table 3). In this study, we identified 4 cases of CML and 3 cases of AML, in which both of these chromosomal abnormalities occurred. Although the prevalence of t(9;22) and inv(16) coexistence has not yet been fully evaluated, a previous study showed that the incidence of t(9;22) in AML with inv(16) is less than 1% (approximately 0.5%) [19]. Our data showed that the coexistence of these abnormalities was detected in 0.6% of CML cases and 2.9% of AML cases with inv(16).
The majority of documented AML patients with t(9;22) and inv(16) coexistence have exhibited M4Eo BM morphology, including an increased number of myelomonocytic cells and abnormal eosinophils with coarse basophilic granules [8]. The AML cases we studied had similar AML-M4Eo BM morphologies. However, because the CML-BP cases in this study also exhibited an increased number of myelomonocytic cells and abnormal eosinophils, we had difficulty in discriminating CML-BP from AML on a morphological basis alone. Patients with a history of CML-CP before the development of a "double positive" can be easily diagnosed with CML-BP. However, we found that patients with AML exhibited a higher number of circulating blasts and more severe BM eosinophilia than did patients with CML-BP.
Cytogenetically, the proportion of each chromosomal abnormality was informative for identifying secondary changes [3]. This study documented a CML patient with secondary inv(16) who also exhibited a minor proportion of a
In most double-positive cases, the major p210 chimeric BCR-ABL1 protein is observed in CML, whereas the minor p190 form correlates with AML presentation. However, some exceptions to this tendency have also been reported [9, 21, 22]. In the present study, a p210 fusion was detected in all patients with CML and 1 patient with de novo AML; moreover, a p190 fusion was detected in the 2 patients with t-AML. These findings suggest that the presence of a p190 BCR-ABL1 fusion protein is associated with AML. In addition, rare
We also analyzed the presence of commonly observed mutations associated with inv(16) and t(9;22). Nacheva et al. [24] have shown that AML with t(9;22) is accompanied by the loss of
De novo AML with coexisting t(9;22) and inv(16) chromosomal abnormalities appears to have a prognosis as favorable as that in AML with inv(16) alone, whereas CML with both t(9;22) and inv(16) seems to have an unfavorable or uncertain prognosis [4, 5]. However, our data show that only 1 patient with CML-BP died of sepsis, and the other patients sustained clinical remission. Imatinib mesylate has been used effectively and safely to treat CML-BP [27]. With the benefits of better tolerance and fewer side effects, it has also been useful as a first-line interim therapy or maintenance strategy to bridge hematopoietic stem cell transplantation in patients with AML [28].
An interesting finding in the present study is that the 2 patients with t-AML exhibited t(9;22) and inv(16) coexistence. Patients with t(9;22) represent 2% of all therapy-related cases of myelodysplastic syndromes and t-AML. Moreover, t(9;22) is significantly associated with previous therapy with topoisomerase II inhibitors [5]. Although inv(16) is a well-known recurrent abnormality in t-AML, it is most frequently observed in patients with breast cancer or lymphoma who have been treated with alkylating agents, topoisomerase II inhibitors, radiation therapy, or a combination thereof. The response rates to intensive antileukemic chemotherapy in patients with t-AML with inv(16) are comparable to those of patients with de novo AML. Overall, 85% of all patients obtain complete remission after intensive chemotherapy [29]. In the present study, 1 patient had follicular lymphoma treated with an alkylating agent, and t-AML occurred 14 months after finishing lymphoma treatment. The other t-AML patient had received chemotherapy including topoisomerase II inhibitors for follicular lymphoma and developed t-AML 10 months after completing treatment. Complex karyotype, reportedly the strongest prognostic indicator, predicts a poor prognosis for t-AML patients. One study has reported that the t-AML M3 phenotype has a good prognosis, but overall survival is significantly shorter in t-AML with a complex karyotype [30].
The present study shows that evaluations of the percentage of circulating blasts and BM eosinophils, careful comparison of initial and follow-up cytogenetics studies including FISH results, and karyotyping of
Table 1 . Patient characteristics..
a)Phase in which cytogenetic studies were performed..
Abbreviations: AML, acute myeloid leukemia; AP, accelerated phase; Bø, basophil; BP, blast phase; CML, chronic myelogenous leukemia; CP, chronic phase; Eø, eosinophil; Hb, hemoglobin; M4Eo, French-American-British Cooperative Group classification M4 with eosinophils; Nø, neutrophil; Plt, platelet; t-AML, therapy-related AML..
Table 2 . Molecular and cytogenetic findings and clinical outcomes..
a)Months from previous diagnosis. b)Months from presence of inv(16) and t(9;22)..
Abbreviations: alloPBSCT, allogeneic peripheral blood stem cell transplant; BM, bone marrow; FISH, fluorescence in situ hybridization; ND, not done; RT-PCR, reverse transcriptase-polymerase chain reaction; uBMT, unrelated BM transplantation; uPBSCT, unrelated peripheral blood stem cell transplant..
Table 3 . Previously reported cases of t(9;22) and inv(16) coexistence..
Abbreviations: AML, acute myeloid leukemia; AML M1, acute myeloblastic leukemia; allo-BMT, allogeneic bone marrow transplant; BP, blast phase; F, female; M, male; m-bcr, minor breakpoint region; M-bcr, major breakpoint region; M4Eo, French-American-British Cooperative Group classification M4 with eosinophils; ND, not done..
Hee Sue Park
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