A Rare Case of Transfusion Transmission of Hepatitis A Virus to Two Patients with Haematological Disease.

BACKGROUND: This paper describes the transmission of hepatitis A virus (HAV) to two blood recipients from a healthy donor that later presented to the blood bank with jaundice. METHODS: The RNA of HAV was detected by qualitative nested reverse transcription polymerase chain reaction (nested RT-PCR) and quantified by real-time RT-PCR. HAV RNA samples were genotyped by direct sequencing of PCR products. A sequence from a fragment of 168 bp from the VP1/2A HAV region was used to construct a phylogenetic tree. CASE REPORT: A 31-year-old male donor accepted for donation of a whole blood unit returned to the blood bank with clinical jaundice 20 days after donation. His serological and NAT tests were negative for HBV and HCV. Serological tests for HAV IgM and IgG were negative on donation sample but positive on follow-up sample, confirming donor's HAV acute infection. Both recipients of red blood cells (R1) and platelet concentrate (R2) from the same implicated donation were HAV IgM-negative and IgG-positive. Qualitative PCR was positive on samples from all three individuals and phylogenetic analysis of viruses proved HAV transmission to the two recipients of blood products. HAV viral load on donor follow-up sample and the platelet recipient was 1.3 and 1.5 × 10(3) IU/ml, respectively. The RBC recipient, also infected by HCV, was undergoing bone marrow transplantation and died from fulminant hepatitis, 26 days after the implicated HAV transfusion. CONCLUSION: The blood donor, a garbage collector, spontaneously returned to the blood bank when developing jaundice. This highlights the importance of donor education to immediately report to blood banks of any signs and symptoms related to infectious disease developed after blood donation. The fact that one immunocompromised patient with HCV infection died from fulminant hepatitis after receiving a HAV-contaminated platelet transfusion underpins the importance of a HAV vaccination program for these group of patients.

Leucemia mieloide aguda: atualidade brasileira de diagnóstico e tratamento / Acute myeloid leukemia: update in diagnosis and treatment in Brazil

Objective: To identify how the Brazilian hematology centers treated and diagnosed cases of acute myeloid leukemia in 2009. Methods: An epidemiological observational multicenter study of 11 listed Brazilian centers that treat acute myeloid leukemia and perform bone marrow transplantation. Data were collected from clinical charts of patients with acute myeloid leukemia treated at the said centers between 2005 and 2009. The availability for immunophenotyping and cytogenetic tests was assessed. Results:During 2009, a total of 345 new cases of acute myeloid leukemia were diagnosed. Differences were noted in the tests performed between patients who initiated treatment at the center and those referred for treatment. Of the participating centers, 72% conducted some type of molecular study in acute myeloid leukemia upon diagnosis. Conclusion: Treatment for acute myeloid leukemia in Brazil shows significantly inferior results when compared to other centers worldwide.

Objetivo: Identificar como centros de hematologia brasileiros trataram e diagnosticaram os casos de leucemia mieloide aguda no ano de 2009. Métodos: Estudo epidemiológico, observacional, multicêntrico de 11 centros brasileiros cadastrados para tratamento de leucemia mieloide aguda e transplante de medula óssea. Os dados foram coletados a partir de prontuários de pacientes com leucemia mieloide aguda tratados nos centros citados entre os anos de 2005 e 2009. Foi avaliada a disponibilidade para realização de exames de imunofenotipagem e citogenética nos centros estudados. Resultados: Foram diagnosticados 345 casos novos de leucemia mieloide aguda no ano de 2009. Observaram-se diferenças na realização de exames entre pacientes que iniciaram o tratamento no centro em relação àqueles referenciados para tratamento. Dos centros participantes, 72% realizaram algum tipo de pesquisa molecular em leucemia mieloide aguda ao diagnóstico. Conclusão: O tratamento da leucemia mieloide aguda no Brasil apresenta resultados muito inferiores quando comparado a outros centros mundiais.

Acute myeloid leukemia: update in diagnosis and treatment in Brazil.

OBJECTIVE: To identify how the Brazilian hematology centers treated and diagnosed cases of acute myeloid leukemia in 2009. METHODS: An epidemiological observational multicenter study of 11 listed Brazilian centers that treat acute myeloid leukemia and perform bone marrow transplantation. Data were collected from clinical charts of patients with acute myeloid leukemia treated at the said centers between 2005 and 2009. The availability for immunophenotyping and cytogenetic tests was assessed. RESULTS: During 2009, a total of 345 new cases of acute myeloid leukemia were diagnosed. Differences were noted in the tests performed between patients who initiated treatment at the center and those referred for treatment. Of the participating centers, 72% conducted some type of molecular study in acute myeloid leukemia upon diagnosis. CONCLUSION: Treatment for acute myeloid leukemia in Brazil shows significantly inferior results when compared to other centers worldwide.

Rapid and sensitive allele-specific (AS)-RT-PCR assay for detection of T315I mutation in chronic myeloid leukemia patients treated with tyrosine-kinase inhibitors.

Point mutations in the kinase domain of BCR-ABL were described in 40-90% of patients with chronic myeloid leukemia (CML) resistant to Imatinib. We herein describe the development of a rapid allele-specific (AS)-RT-PCR assay to identify the T315I mutation, which confers full resistance to all available tyrosine-kinase inhibitors (TKI). The mutation status of 65 patients with resistant CML was evaluated, and the T315I was detected in 3/65 (4.6%). Comparisons between sequencing and AS-RT-PCR results, as well as serial dilutions experiments proved that the method is specific and reproducible, with maximum sensitivity of 1 × 10(-3). The developed assay is a convenient and easy tool to be used in research of CML resistance for rapid mutation screening and, together with sequencing, may be included in efficient strategies for early detection of TKI resistance in patients with CML.

Epigenetic alterations of p15(INK4B) and p16(INK4A) genes in pediatric primary myelodysplastic syndrome.

We studied the methylation status of the p15(INK4B) and p16(INK4A) genes in 47 pediatric patients with primary MDS, its correlation with subtype, and the role of p15(INK4B) and p16(INK4A) in the evolution of MDS toward AML. Aberrant methylation of the p15(INK4B) gene was detected in 15 of 47 patients (32%), whereas only four patients demonstrated methylation of the p16(INK4A) gene (8%). The frequency of p15(INK4B) methylation was significantly higher in RAEB and RAEB-t subtypes (p<0.003). Aberrant methylation of the p16(INK4A) gene was also more frequent in the subtypes that characterize advanced stages of the disease (p<0.05). Evolution of disease was verified in 17 (36%) of the 47 patients. The association of p15(INK4B) and p16(INK4A) methylation status with evolution of disease was clearly significant (p<0.008 and p<0.05, respectively). These results suggest that methylation of the p15(INK4B) and p16(INK4A) genes is an epigenetic biomarker of pediatric disease evolution.

Benefits of the intermittent use of 6-mercaptopurine and methotrexate in maintenance treatment for low-risk acute lymphoblastic leukemia in children: randomized trial from the Brazilian Childhood Cooperative Group--protocol ALL-99.

PURPOSE To describe event-free survival (EFS) and toxicities in children with low-risk acute lymphoblastic leukemia (ALL) assigned to receive either continuous 6-mercaptopurine (6-MP) and weekly methotrexate (MTX) or intermittent 6-MP with intermediate-dose MTX, as maintenance treatment. PATIENTS AND METHODS Between October 1, 2000, and December 31, 2007, 635 patients with low-risk ALL were enrolled onto Brazilian Childhood Cooperative Group for ALL Treatment (GBTLI) ALL-99 protocol. Eligible children (n = 544) were randomly allocated to receive either continuous 6-MP/MTX (group 1, n = 272) or intermittent 6-MP (100 mg/m(2)/d for 10 days, with 11 days resting) and MTX (200 mg/m(2) every 3 weeks; group 2, n = 272). RESULTS The 5-year overall survival (OS) and EFS were 92.5% +/- 1.5% SE and 83.6% +/- 2.1% SE, respectively. According to maintenance regimen, the OS was 91.4% +/- 2.2% SE (group 1) and 93.6% +/- 2.1% SE (group 2; P = .28) and EFS 80.9% +/- 3.2% SE (group 1) and 86.5% +/- 2.8% SE (group 2; P = .089). Remarkably, the intermittent regimen led to significantly higher EFS among boys (85.7% v 74.9% SE; P = .027), while no difference was seen for girls (87.0% v 88.8% SE; P = .78). Toxic episodes were recorded in 226 and 237 children, respectively. Grade 3 to 4 toxic events for groups 1 and 2 were, respectively, 273 and 166 for hepatic dysfunction (P = .002), and 772 and 636 for hematologic episodes (P = .005). Deaths on maintenance were: seven (group 1) and one (group 2). CONCLUSION The intermittent use of 6-MP and MTX in maintenance is a less toxic regimen, with a trend toward better long-term EFS. Boys treated with the intermittent schedule had significantly better EFS.

SUZ12 is a candidate target of the non-canonical WNT pathway in the progression of chronic myeloid leukemia.

Polycomb proteins form multiprotein complexes that repress target genes by chromatin remodeling. In this work, we report that the SUZ12 polycomb gene is over-expressed in bone marrow samples of patients at the blastic phase of chronic myeloid leukemia. We also found a direct interaction between polycomb group genes and the WNT signaling pathway in chronic myeloid leukemia transformation. Electrophoretic mobility shift assay (EMSA), Chromatin immunoprecipitation assay (ChIP), and mass spectrometry assays identified noncanonical WNT pathway members, such as WNT5A and WNT11, bound to the SUZ12 promoter. Immunohistochemistry and immunofluorescence with WNT5A and WNT11 antibodies confirmed nuclear localization. Knockdown of WNTs 1, 5A, and 11 with RNAi approaches showed that WNT members are capable of activating SUZ12 transcription with varying promoter affinities. Finally, we suggest that SUZ12 is blocking cellular differentiation, as SUZ12 knockdown release differentiation programs in chronic myeloid blastic phase (CML-BP) transformed cell line.

Burkitt lymphoma/leukaemia transformed from a precursor B cell: clinical and molecular aspects.

Burkitt lymphoma/leukaemia (BL/L) is a heterogeneous disease with respect to epidemiological patterns and cell origin. The occurrence of BL/L with an immature phenotype raises the question whether this phenotype might be a consequence of early B-cell transformation or, alternatively, a secondary feature of transformed, mature B cells. It also poses important clinical questions regarding diagnosis and therapeutic procedures. Here we describe the case of a 4-yr-old child with BL/L and FAB L3 morphology, with phenotypic and genotypic characteristics of a CD10+ precursor B-cell acute lymphoid leukaemia (ALL) associated with t(8;14)(q24;q32). Molecular analysis showed expression of RAG1 and RAG2 and an unmutated VDJCmu immunoglobulin rearrangement coinciding with a lack of AICDA expression, indicating an immature B-cell origin. His clinical response suggested that FAB L3 ALL with MYC rearrangement and an aberrant precursor B-cell phenotype is clinically similar to BL/L. Moreover, short, intensive chemotherapeutic protocols seemed to be beneficial. This case also allowed us to refine the description of cellular and molecular variants of BL/L regarding the cell origin and pathogenesis of this biologically heterogeneous disease.

The impact of addictional chromosomal abnormalities in response to imatinib mesylate therapy for chronic myeloid leukemia

Imatinib induces a complete cytogenetic response in more than 80% of newly diagnosed patients with chronicmyeloid leukemia (CML) in the chronic phase (CP) and in 41% of patients in the first chronic phase after failureof interferon- treatment. However, some patients do not respond completely. Therefore, according to moststudies, drug resistance in CML patients treated with imatinib is correlated with cytogenetic abnormalities acquiredduring treatment. In this study we analyzed 48 CML patients treated with imatinib mesylate after interferon- resistance in order to elucidate the impact of additional chromosomal abnormalities prior to imatinib in response to therapy. Cytogenetic abnormalities in addition to the Philadelphia chromosome (Ph) were detected in 33.3% of patients. Patients with Ph as the sole cytogenetic abnormality prior to imatinib therapy presented a major cytogeneticresponse and significantly longer median overall survival (p=0.006) than patients with additional chromosomalabnormalities. Therefore, in this group of patients, another choice of treatment should be considered, such as stemcell transplantation or combination regimens as appropriate. The present study indicates the importance of detecting a double Ph chromosome prior to imatinib therapy. Patients showing this abnormality did not respond to imatinib, thus indicating the abnormality's association with resistance. Our study suggests that classical cytogenetic analysisis still an important tool prior to and during follow-up of CML patients treated with imatinib.

Imatinibe induz à resposta citogenética completa em cerca de 80 por cento dos pacientes diagnosticados com leucemia mielóide crônica (LMC) em fase crônica (FC), e em 41 por cento dos pacientes em primeira FC após falha do tratamento com interferon-alfa. Alguns pacientes, entretanto, não respondem completamente. Em muitos estudos, a resistência à droga em pacientes tratados com imatinibe é correlacionada a alterações cromossômicas adquiridas durante o tratamento. No presente estudo, foram analisados 48 pacientes tratados com imatinibe após resistência ao interferon-alfa, com o objetivo de verificar o impacto das alterações cromossômicas adicionais ao Philadelphia (Ph), prévias à terapia com imatinibe. Alterações adicionais foram detectadas em 33,3 por cento dos pacientes. Pacientes com somente o cromossomo Ph apresentaram melhor taxa de resposta citogenética e sobrevida global significativa maior quando comparados com os pacientes que apresentavam alterações cromossômicas adicionais antes do início da terapia com imatinibe. Assim, nesse grupo de pacientes, a escolha de outra conduta terapêutica, como o transplante de células tronco-hematopoéticas ou regime de combinação de drogas, pode ser indicada. O presente estudo indica a importância do duplo Ph antesdo início da terapia com imatinibe. Todos os pacientes com esta alteração não responderam ao tratamento, sendo a mesma associada à resistência à droga. Este estudo sugere que a citogenética clássica permanece como uma ferramenta importante no monitoramento de pacientes portadores de LMC tratados com imatinibe.

Uso simultâneo do método do polimorfismo conformacional de fita simples e da citometria de fluxo no aumento da eficácia da detecção de anormalidades do gene e da proteína p53 na leucemia mielóide crônica / Simultaneous use of the single strand conformation polymorphism method and flow cytometry for increasing the detection efficacy of abnormalities in the gene and p53 protein in chronic myeloid leukemia

A proteína p53 desempenha um importante papel no controle do ciclo de celular e reparo no DNA danificado. Em pacientes com leucemia de mielóide crônica (LMC) as mutações neste gene são encontradas em até 30% dos casos, especialmente na crise blástica (LMC-CB), sendo a detecção de alterações nesse gene ou proteína importantes na avaliação da evolução clínica da LMC. O sequenciamento de DNA é descrito como o método capaz de identificar as mutações do gene TP53, sendo, no entanto uma técnica complexa e dispendiosa, o que dificulta seu emprego em larga escala, sendo, atualmente, proposto a pesquisa da proteína p53 por métodos imunológicos e a técnica da reação em cadeia da polimerase seguida pelo estudo do polimorfismo conformacional de fita simples (PCR/SSCP). Métodos: Analisaram-se amostras de 72 pacientes com LMC: 54 de LMC em fase crônica (33 fase inicial ou LMC-FCi e 21 em fase crônica tardia ou LMC-FCtd), 7 em fase acelerada ou LMC-Ac e 11 em crise de blástica (LMC-CB). Foram realizados PCR para os exons 5-9 para posterior estudo pelo SSCP e a expressão de proteína de p53 foi feita por citometria de fluxo. Resultados: Na análise do PCR-SSCP, alterações de mobilidade eletroforética indicativa de mutação do gene de TP53 foi observado em 11/72 pacientes e a expressão da proteína p53 em 17/72 pacientes. O SSCP anormal foi visto em dois casos de LMC-FCi (exon 7), quatro LMC-FCt (um exon 7, um exon 8 e dois exons 8-9), um na LMC-FAc (exon 8) e quatro na LMC-CB (dois no exon 5, um no exon 6 e um no exon 8-9). Neste grupo, a proteína de p53 estava expressa sete casos (todas LMC-CB e AC e 2 LMC-FCtd), havendo correlação estatisticamente significativa entre os resultados dos dois métodos. Conclusões: Estes resultados sugerem que os dois métodos conjuntamente empregados podem aumentar a sensibilidade na detecção de anormalidades do gene e proteína p53 nos pacientes com LMC. A presença de SSCP anormal associado à expressão da proteína de p53 nas fases avançadas desta doença na maioria de casos, sugere que estes exames possam se empregados como indicadores de progressão para a LMC.

The p53 protein play an important role in the control of the cell cycle and DNA repair. In patients with chronic myeloid leukemia (CML) mutation in this gene were found in up to 30%, especially among those in blast crisis. At present, the only widely available technology that reliable detects and defines all mutations is DNA sequencing. However, the routine sequencing of the entire TP53 gene in all cases suggestive of mutation in the laboratorial routine is prohibitively costly, complex, and time consuming. To screen for TP53 abnormalities in CML patients, both p53 protein expression bay immunologic methods and single strand conformation polymorphism of polymerase chain reaction products (SSCP-PCR) is proposed. Methods: We report the results of an analysis of 72 samples from CML patients:54 in chronic phase :33 in initial phase (ICP-CML) and 21 in late phase (LCP-CML), 7 in accelerated phase (AP-CML) and 11in blast crisis (BC-CML). DNA structure for 5-9 exons of the TP53 gene were analyzed by PCR-SSCP and p53 protein expression by flow cytometry (CF). Results: By PCR-SSCP analysis, shifts in eletrophoretic mobility of the TP53 gene were detected in 11 out of CML patients and p53 protein expression in 17 out of 72 CML patients. The abnormal SSCP pattern were showed in two cases of ICP-CML (exon 7), four LCP-CML (one exon 7 and exon 8 and two exons 8-9), one in AP-CML (exon 8) and four in BC-CML (two in exon 5, one in exon 6 and one in exon 8-9). In this group, the p53 protein were express in 17 cases (all CB and AC of CML patients and 2 out of 5 LCP samples of CML patients) and the statistical analysis by qui-square test showed correlation between this two tests. Conclusions: These results suggest that the two methods together can increase the sensibility of screening for p53 abnormalities in CML patients. The presence of abnormal SSCP associated to the p53 protein expression in advanced phases of this disease in the most of cases, suggesting that these tests can be used as an indicator of progression of CML.

Detecção da proteína p53 em células leucêmicas por citometria de fluxo e imunocitoquímica / Detection of p53 protein in leukemic cells by flow cytometry and immunocytochemistry

Introdução: A proteína p53 desempenha uma função crucial no controle do ciclo celular, reparo do DNA e na indução de apoptose em células geneticamente instáveis. A imunocitoquímica (ICQ) é um dos métodos preconizados para detecção e visualização dessa proteína no núcleo das células, sendo, no entanto um método demorado e trabalhoso o que dificulta a sua aplicação na rotina laboratorial. Atualmente, a citometria de fluxo (CF) também tem sido empregada na detecção da proteína p53 mutada ou estabilizada tendo a vantagem da praticidade e rapidez de execução. Objetivos e Metodologia: Comparar os resultados obtidos pela CF e ICQ na detecção da proteína p53 em células leucêmicas. Empregamos amostras de 10 pacientes com leucemia linfóide aguda (LLA) 10 com leucemia linfóide crônica (LLC), tendo sido também empregadas, células de linhagens leucêmicas humanas que serviram como controle de expressão positiva e negativa para ambos os métodos além de linfócitos de 40 doadores de sangue. A CF e ICQ foram realizadas após a marcação com anticorpo monoclonal anti-p53 por técnicas convencionais. Resultados: Observamos concordância nos resultados da maioria das amostras dos pacientes e em todas as amostras das linhagens elulares tendo sido, no entanto constatados níveis de expressão mais elevados nas análises obtidos pela CF quando comparados com a ICQ, refletindo em uma maior sensibilidade desse método. Conclusão: Apesar da ICQ ser considerada uma técnica adequada para a detecção da p53, nossos resultados indicam que a CF pode ser empregada satisfatoriamente na detecção dessa proteína em amostras de células leucêmicas.

Introduction: The p53 protein plays a crucial role in the cell cycle control, DNA damage repair and induction of apoptosis in genetically unstable cells. The immunocytochemistry (ICQ) is one of the most common methodology for detection and visualization of this protein in the nucleus of the cells, but this technique is time-consuming and difficult to apply in the clinical setting. Nowadays the assessment of p53 protein expression by flow cytometry (FC) assays are easier to perform and provide reliable estimates of the prolonged half-life of mutant or inactivated wild-type p53 protein. Objectives and Methodology: Compare the results of p53 detection by FC and ICQ in leukemic cells. We used samples from 10 patients with acute lymphoid leukemia (ALL), 10 with chronic lymphoid leukemia (CLL). To positive and negative controls of p53 expression in both methods we also employed leukemic cells from human leukemic cell lines an lymphocytes from 40 healthy donors were also used as control for negative labeling in FC. The FC and ICQ were performed after labeling with p53 monoclonal antibody by the usual protocol. Results: We verified an agreement in the results in the majority of the leukemic cells from patients and in all human leukemic cell line samples. Conclusion: Despite of ICQ is considered a good methodology for p53 detection in leukemic cells; our results show that FC can be satisfactorily used for detection of this protein in leukemic cells.

Transformação da LLC-B: síndrome de Richter / Transformation of the CLL-B: Richter's syndrome

A síndrome de Richter é caracterizada pela transformação da leucemia linfóide crônica (LLC) para o linfoma não-Hodgkin de alto grau de malignidade, leucemia pró-linfocítica, doença de Hodgkin, mieloma múltiplo ou leucemia linfoblástica. A transformação de Richter ocorre em 2 por cento-6 por cento dos casos de LLC, mas a incidência pode ser maior, se nova biópsia de linfonodo for realizada no paciente com alterações clínicas, mas com leucemia previamente controlada. A despeito do tratamento agressivo, a duração da sobrevida mediana varia de 5 a 8 meses. Logo, novas estratégias visando ao tratamento curativo são necessárias.

Richter's Syndrome denotes the leukemic evolution to high-grade non-Hodgkin's lymphoma, prolymphocytic leukemia, Hodgkin's disease, multiple myeloma or acute lymphoblastic leukemia in patients with chronic lymphocytic leukemia (CLL). Richter's syndrome occurs in 2 percent to 6 percent of all cases of CLL, but the incidence may be higher if lymph node biopsies are performed when systemic symptoms develop in patients with previously well-controlled leukemia. Current treatments are aggressive, but prognosis is poor, and the median survival ranges from five months to eight months. Thus, novel curative treatment strategies are needed.

Biological diversity variations of pediatric acute leukemia in Brazil: contribution of immunophenotypic profiles to epidemiological studies

Os autores descrevem as características biológicas de 1.459 crianças com leucemias agudas no Brasil, para comparar os efeitos de diferentes perfis imunofenotípicos com fatores ambientais que podem estar associados à etiologia das leucemias linfoblásticas agudas (LLA). As classificações morfológicas e imunofenotípicas combinadas foram aplicadas em 96% dos casos. Nestes, 55% foram classificados como LLA de células B precursoras (LLA-Bp) que compreendem LLA-pro-B e LLA-comum, 15% LLA-T, e 1,6% LLA-B. A proporção de LLA-Bp e LLA-T difere entre si quanto à raça, com 59% das LLA-Bp em crianças brancas, enquanto 60,7% LLA-T em crianças não-brancas. No entanto, as análises proporcionais de brancos versus não brancos para cada subtipo, quando ajustadas por idade, são semelhantes em crianças maiores de 6 anos (60,3% LLA-Bp e 59,3% LLA-T), mas diferem substancialmente em crianças menores, com 63,6% de LLA-Bp e 37,3% de LLA-T em brancos (0,0001). Estes resultados são consistentes com excesso de LLA-Bp em crianças brancas mais jovens, embora a distribuição entre LLA-Bp e LLA-T em cada região seja semelhante sem significado estatístico. As taxas de incidências de LLA calculadas para cada região variaram de 2,2, 2,6 e 3,3/105 casos por ano para Bahia, Rio de Janeiro e Brasília, respectivamente. Para avaliar se o pico de incidência observado de LLA-Bp estaria relacionado com incidência de infeção viral, nós observamos que LLA-Bp apresentou uma curva ascedente de casos no verão e inverno, enquanto LLA-T apresentou pico de incidência no outono. Este estudo adiciona informações sobre epidemiologia de leucemias agudas no Brasil, no qual sugere que o subtipo LLA-comum poderia estar associado com tempo de exposição a infecção viral requerendo futuras análises específicas.

Coexpression of p53 protein and MDR functional phenotype in leukemias: the predominant association in chronic myeloid leukemia.

BACKGROUND: One of the best characterized resistance mechanisms of leukemias is multidrug resistance (MDR) mediated by P-glycoprotein (Pgp) and multidrug-resistant related protein (MRP). In addition to Pgp and MRP, p53 mutation or inactivation might play a relevant role in therapeutic failure. Some studies have demonstrated that Pgp and MRP may be activated in association with overexpression of mutant or inactivated p53 protein. The aim of this study was to investigate the association between p53 expression and MDR functional phenotype analyzed by flow cytometry (FCM). METHODS: Rhodamine-123 assay analyzed by FCM was used to detect the MDR phenotype that was positive in 18 out of 41 (43.9%) cases of chronic myeloid leukemia (CML), 16 out of 28 (57.1%) chronic lymphoid leukemia (CLL) cases, 11 out of 28 (39.3%) acute myeloid leukemia (AML) cases, and four out of 22 (18.2%) acute lymphoid leukemia (ALL) cases. RESULTS: Variable levels of p53 expression were observed in leukemic cells: 12 out of 41 (29.2%) in CML, nine out of 28 (32.1%) in CLL, 15 out of 28 (53.6%) in AML, and eight out of 22 (36.4%) in ALL samples. CONCLUSIONS: In our study, no significant association between p53 expression and MDR functional phenotype was observed in ALL, CLL, and AML. On the other hand, a significant association (P = 0.0003) of the coexpression was observed in CML. The p53 overexpression was more frequently seen in the accelerated phase and the blastic phase of this disease. Our results suggest that an MDR functional phenotype could be associated with p53 mutation in the advanced stage of leukemias.