Clinical characteristics and prognostic implications of NPM1 mutations in acute myeloid leukemia

doi:10.1182/blood-2005-04-1733

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Blood, 15 October 2005, Vol. 106, No. 8, pp. 2854-2861.
Prepublished online as a Blood First Edition Paper on June 30, 2005; DOI 10.1182/blood-2005-04-1733.

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NEOPLASIA
Clinical characteristics and prognostic implications of NPM1 mutations in acute myeloid leukemia
Tatsuya Suzuki, Hitoshi Kiyoi, Kazutaka Ozeki, Akihiro Tomita, Satomi Yamaji, Ritsuro Suzuki, Yoshihisa Kodera, Shuichi Miyawaki, Norio Asou, Kazutaka Kuriyama, Fumiharu Yagasaki, Chihiro Shimazaki, Hideki Akiyama, Miki Nishimura, Toshiko Motoji, Katsuji Shinagawa, Akihiro Takeshita, Ryuzo Ueda, Tomohiro Kinoshita, Nobuhiko Emi, and Tomoki Naoe
From the Department of Infectious Diseases and the Department of Hematology, Nagoya University Graduate School of Medicine, Nagoya; Division of Molecular Medicine, Aichi Cancer Center, Nagoya; Department of Medicine, Japanese Red Cross Nagoya First Hospital, Nagoya; Department of Medicine, Saiseikai Maebashi Hospital, Maebashi; Department of Hematology, Kumamoto University School of Medicine, Kumamoto; Department of Hematoimmunology, School of Health Sciences, Faculty of Medicine, University of the Ryukyus, Nishihara; Department of Internal Medicine (Hematology), Saitama Medical School, Saitama; Division of Hematology and Oncology, Department of Medicine, Kyoto Prefectural University of Medicine, Kyoto; Department of Hematology, Tokyo Metropolitan Komagome Hospital, Tokyo; Second Department of Internal Medicine, Chiba University School of Medicine, Chiba; Department of Hematology, Tokyo Women's Medical University, Tokyo; Second Department of Internal Medicine, Okayama University School of Medicine, Okayama; Department of Medicine III, Hamamatsu University School of Medicine, Hamamatsu; and Department of Internal Medicine and Molecular Science, Nagoya City University School of Medicine, Nagoya, Japan.

   Abstract

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Recently, somatic mutations of the nucleophosmin gene (NPM1),which alter the subcellular localization of the product, havebeen reported in acute myeloid leukemia (AML). We analyzed theclinical significance of NPM1 mutations in comparison with cytogenetics,FLT3, NRAS, and TP53 mutations, and a partial tandem duplicationof the MLL gene (MLL-TD) in 257 patients with AML. We foundNPM1 mutations, including 4 novel sequence variants, in 64 of257 (24.9%) patients. NPM1 mutations were associated with normalkaryotype and with internal tandem duplication (ITD) and D835mutations in FLT3, but not with other mutations. In 190 patientswithout the M3 French-American-British (FAB) subtype who weretreated with the protocol of the Japan Adult Leukemia StudyGroup, multivariate analyses showed that the NPM1 mutation wasa favorable factor for achieving complete remission but wasassociated with a high relapse rate. Sequential analysis using39 paired samples obtained at diagnosis and relapse showed thatNPM1 mutations were lost at relapse in 2 of the 17 patientswho had NPM1 mutations at diagnosis. These results suggest thatthe NPM1 mutation is not necessarily an early event during leukemogenesisor that leukemia clones with NPM1 mutations are sensitive tochemotherapy. (Blood. 2005;106:2854-2861)

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Acute myeloid leukemia (AML) is characterized by autonomousproliferation and impaired differentiation of hematopoieticprogenitors but is a genetically and phenotypically heterogeneousdisease. A number of genetic mutations, such as point mutations,gene rearrangements, and chromosomal translocations, which areinvolved in the pathogenesis of leukemia, have been documented.Recently, it was suggested that AML is the consequence of 2broad complementation classes of mutations: those that confera proliferative or a survival advantage to hematopoietic progenitors(class 1)—including activating mutations in tyrosine kinasessuch as BCR-ABL1, ETV6-PDGFRB, KIT, and FLT3 or their downstreameffectors such as NRAS—and those that impair hematopoieticdifferentiation and confer properties of self-renewal (class2)—including rearrangements or point mutations of corebinding factor (CBF) genes and PML-RARA.¹ Mutations in FLT3,NRAS, and KIT have been found in approximately 30% to 35%, 15%to 20%, and 5% to 10% of adult patients with AML, respectively,indicating that mutations in these 3 genes are the most frequentgenetic alterations in AML.^2-12 FLT3 and KIT mutations are oftenfound in AML patients with PML-RARA and CBF gene translocations,respectively,^13,14 whereas FLT3 mutations have been preferentiallyfound in AML patients with normal karyotype. Because mutatedFLT3 reportedly induces myeloproliferative disease (MPD), butnot AML, in primary hematopoietic progenitors in the murinebone marrow transplantation model and MPD does not have serialtransplantability, FLT3 mutations alone are not sufficient forthe development of AML.¹⁵ Therefore, it has been suggested thatadditional mutations are involved in the pathogenesis of AMLwith FLT3 mutations.
Recently, Falini et al¹⁶ reported that the nucleophosmin gene(NPM1) is mutated in a high proportion of adults with AML, resultingin an aberrant cytoplasmic localization of the product (NPMc+).Of note is that NPMc+ is associated with a wide spectrum ofmorphologic subtypes of AML, a normal karyotype, and FLT3 mutations.Furthermore, NPMc+ AML is clinically associated with betterresponsiveness to induction chemotherapy, although its prognosticimplications for long-term outcome remain unclear. Althoughthe prevalence and significance of several genetic abnormalitiesin patients with AML have been reported to date, the most powerfulprognostic factor in AML has been the karyotype of the leukemiacells.¹⁷ Three cytogenetic risk groups (favorable, intermediate,and poor) are widely accepted, but there is a practical limitationto the definition of cytogenetic risk, especially in patientsin the intermediate group. Additional prognostic factors are,therefore, required. We and several groups^9,10,12,18 have demonstratedthat FLT3 mutations are a strong prognostic factor in AML, especiallyin patients with normal karyotype, but they do not affect responsivenessto induction chemotherapy. Therefore, NPM1 mutations seem tocharacterize a distinct disease entity not only of AML withnormal karyotype but also of AML with FLT3 mutations.
NPM is a ubiquitously expressed phosphoprotein, continuouslyshuttles between the nucleus and the cytoplasm,^19,20 and isinvolved in the oncogenesis of some types of leukemia and lymphomabecause the NPM gene is a partner in several tumor-associatedchromosomal translocations.^21-23 However, it is also thoughtto have a tumor-suppressor function and to regulate the p53pathway through its chaperoning activity.^24-26 It is suggestedthat a loss of nuclear NPM function caused by mutation mightimpair the p53 pathway and that a lack of p53 might induce geneticinstability²⁷; hence, NPM1 mutations seem to cause AML cellsto acquire additional genetic alterations.
In this study, we analyzed the prevalence and clinical characteristicsof NPM1 mutations in comparison with cytogenetics, FLT3, NRAS,and TP53 mutations and a partial tandem duplication of the MLLgene (MLL-TD) in 257 patients with newly diagnosed de novo AML.The prognostic implications of NPM1 mutations were evaluatedin 190 patients with AML, excluding those with the M3 FAB subtype,who were treated according to the protocol of the Japan AdultLeukemia Study Group (JALSG). Furthermore, to clarify the stabilityof NPM1 mutations and the potential effect on genetic instabilityin AML cells during disease progression, we compared the mutationalstatus of these genes in 39 paired samples obtained at initialdiagnosis and first relapse.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patients and samples
The diagnosis of AML was based on the French-American-British(FAB) classification. The study population included 257 patientswith newly diagnosed de novo AML, as follows: 9 with the M0,54 with the M1, 89 with the M2, 15 with the M3, 54 with theM4, 19 with the M5, 8 with the M6, and 9 with the M7 FAB subtype.In 39 of the 257 AML patients, paired samples obtained at diagnosisand first relapse were available. Furthermore, in 6 patients,samples obtained at diagnosis and complete remission (CR) wereavailable. Bone marrow (BM) samples from patients with AML weresubjected to Ficoll-Hypaque (Pharmacia LKB, Uppsala, Sweden)density gradient centrifugation. All samples taken at diagnosisor relapse were confirmed to contain more than 90% leukemiacells after enrichment by centrifugation. Informed consent wasobtained from all patients to use their samples for bankingand molecular analysis, and approval for these studies was obtainedfrom the Nagoya University institutional review board.
Cytogenetic G-banding analysis was performed according to standardmethods. In this study, cytogenetic risk groups were stratifiedaccording to the criteria adopted by the Medical Research Council.²⁸
Screening for mutations of the FLT3, NRAS, and TP53 genes and of MLL-TD
High molecular weight DNA and total RNA were extracted fromthe samples using standard methods. FLT3 gene mutations of theITD (FLT3/ITD) and activation loop (FLT3/D835Mt), NRAS genemutations of codons 12, 13, and 61, and TP53 gene mutationsof exons 5 to 8 were examined as reported and were confirmedby the sequencing procedure.^4,29,30 MLL-TD was examined by reversetranscription-polymerase chain reaction (RT-PCR), as describedpreviously.³¹
Screening for mutations of the NPM1 gene
For the screening of NPM1 mutations, we amplified genomic DNAcorresponding to exon 12 of NPM1 by PCR using the primers NPM1-F,5'-TTAACTCTCTGGTGGTAGAATGAA-3' and NPM1-R, 5'-CAAGACTATTTGCCATTCCTAAC-3',as previously reported.¹⁶ Amplified products were separatedthrough agarose gel, purified using a QIAquick gel extractionkit (Qiagen Inc, Chatsworth, CA), and directly sequenced ona DNA sequencer (310; Applied Biosystems, Foster City, CA) usinga BigDye terminator cycle sequencing kit (Applied Biosystems).If mutations were found by direct sequencing, the fragmentswere cloned into a pGEM-T Easy vector (Promega, Madison, WI),then transfected into the Escherichia coli strain DH5 ${alpha}$ . At least4 recombinant colonies were selected, and plasmid DNA was preparedusing a QIAprep Spin Miniprep Kit (Qiagen Inc) and sequenced.
Analysis of clinical characteristics
It was necessary to analyze the clinical characteristics ina well-documented group. Among the 257 patients analyzed, 15had acute promyelocytic leukemia (APL). APL has been considereda separate disease entity among AML, and the introduction ofall-trans retinoic acid (ATRA) has dramatically improved itsclinical outcome.³² In addition, 52 patients with AML, excludingthose with APL, were treated with independent regimens. We,therefore, analyzed the clinical characteristics of 190 patientswith AML, excluding those with APL, who were treated with theAML87, AML89, and AML92 protocols of JALSG.^33-35 (Each protocolis presented in Document S1; see the Supplemental Document linkat the top of the online article, at the Blood website.)
Statistical analysis
Differences in continuous variables were analyzed using theMann-Whitney U test for distribution between 2 groups. Analysisof frequencies was performed using the Fisher exact test for2 x 2 tables or the Pearson ${chi}$ ² test for larger tables. Multivariateanalysis to identify risk factors for achieving CR was performedusing the logistic regression model. Survival probabilitieswere estimated by the Kaplan-Meier method, and differences insurvival distributions were evaluated using the log-rank test.Overall survival was defined as the time from the first dayof therapy to death or last visit. Relapse-free survival wasdefined as the time from the first day of CR to relapse, death,or last visit. Patients undergoing hematopoietic stem cell transplantationwere censored at the time of transplantation. The prognosticsignificance of the clinical variables was assessed using theCox proportional hazards model. These statistical analyses wereperformed with StatView-J 5.0 (Abacus Concepts Inc, Berkeley,CA). For all analyses, the P values were 2-tailed, and P <.05 was considered statistically significant.

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

NPM1 mutations were frequently found in AML
We first screened for mutations within exon 12 of the NPM1 genethrough direct sequencing in 257 patients with AML, then confirmedeach type of mutation by cloning. We found the NPM1 mutationin 64 of 257 (24.9%) patients (Table 1). Importantly, directsequencing revealed that all AML cells with NPM1 mutations retainedthe wild-type allele. Given that all samples contained morethan 90% AML cells, all mutations seemed to occur in only oneallele. Previously, 6 kinds of mutants, designated mutationsA to F, were identified. In this study, we found 49 mutationsof type A, 7 mutations of type B, 4 mutations of type D, and4 novel mutants that were designated mutations G to J (Figure 1).All novel mutations included distinct 4-bp insertions (mutationG, TTTG; mutation H, CTTG; mutation I, TAAG; mutation J, TATG)at position 960, resulting in the same frameshift as mutationsA to D. Predicted mutant proteins of mutations G and H and ofmutation J were the same as those of mutations A and B, respectively.The protein of mutation I contained a lysine residue at position289, although the other residues were conserved.

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Table 1.. Relationship among NPM1 mutation, FAB type, and genetic alterations in AML

In 2 patients whose leukemia cells had NPM1 mutations at diagnosis,the mutations were lost at CR, indicating that these were somaticmutations.
Morphologic and genotypic characteristics of AML with NPM1 mutations
NPM1 mutations were found in patients with AML of all FAB subtypesexcept M3 (Table 1). Cytogenetic data were available for 209patients. Consistent with findings of a previous report,¹⁶ theNPM1 mutation was preferentially found in patients with normalkaryotype (46 of 97; 47.4%), but it was not found in patientswith t(8;21), t(15;17), del(5), or del(7). In total, there wasa significant difference in the frequency of the NPM1 mutationamong patients with (7 of 112; 6.3%) and without (46 of 97;47.4%) cytogenetic abnormalities (P < .001). Moreover, anNPM1 mutation was found in each of 8 and 3 patients with inv(16)and t(9;22), respectively.
FLT3/ITD and FLT3/D835Mt were found in 58 (22.6%) and 9 (3.5%)of 257 patients, respectively (Table 1). Both FLT3 mutationswere significantly associated with NPM1 mutations: 35 of 58(60.3%) FLT3/ITD (P < .001) and 4 of 9 (44.4%) FLT3/D835Mt(P = .028) were found in the patients with NPM1 mutations. TP53,NRAS, and MLL-TD mutations were found in 16 of 243 (6.6%), 34of 236 (14.4%), and 17 of 147 (11.6%) patients, respectively,although there was no significant correlation between thesemutations and the NPM1 mutation (Table 1).
Clinical characteristics and prognoses of AML patients with or without NPM1 mutations
Among the 257 patients with AML, 190 patients (excluding thosewith M3 who were treated with the AML87, AML89, and AML92 protocolsof the JALSG) were evaluated for clinical characteristics andinitial response to therapy (Table 2). Of these patients, 49(25.8%) had NPM1 mutations. The presence of NPM1 mutations wasrelated neither to sex nor to the occurrence of hepatosplenomegalyor extramedullary involvement. Patients with NPM1 mutations(median, 58 years; range, 15-77 years) were significantly olderthan those without mutations (median, 47 years; range, 15-85years) (P = .003). White blood cell (WBC) counts and peripheralblood blast cells were significantly higher in the NPM1 mutationgroup than in the wild-type group (P = .002 and P = .029, respectively).According to the FAB classification, the NPM1 mutation was infrequentin the M2 subtype (P = .004). According to the cytogenetic riskgroups, the NPM1 mutation was preferentially found in the intermediaterisk group (P < .001). NPM1 mutations were associated withFLT3/ITD (P < .001) and FLT3/D835Mt (P = .018), but not withTP53 and NRAS mutations. Because we could analyze MLL-TD inonly 118 of the 190 patients, we excluded MLL-TD from the variablesfor statistical analysis.

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Table 2.. Characteristics of 190 patients with AML, excluding patients with the M3 subtype, treated according to JALSG protocols

Of the 190 patients, 139 (73.2%) achieved CR after inductionchemotherapy. The CR rate was significantly higher in the patientswith NPM1 mutations (42 of 49; 85.7%) than without them (97of 141; 68.8%) (P = .025). In addition, Fisher exact test showedthat FAB subtypes other than M2, cytogenetic findings otherthan good risk, and the presence of NRAS and TP53 mutationswere unfavorable factors for achieving CR (P < .001, P =.002, P = .030, and P = .034, respectively). Age (older than60), WBC count (more than 100 x 10⁹/L), and presence of theFLT3 mutation were not associated with the CR rate. Multivariatelogistic regression analysis showed that wild-type NPM1 (P <.001), FAB subtypes other than M2 (P = .008), and cytogeneticfindings other than good risk (P = .039) were independent unfavorablefactors for achieving CR (Table 3).

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Table 3.. Logistic regression analysis results of the effect of unfavorable factors for CR in 190 patients, excluding those with the M3 subtype, treated according to JALSG protocols

Kaplan-Meier analyses according to NPM1 mutation are shown inFigure 2A. Univariate analysis showed that the poor prognosticfactors for overall survival were age 60 or older (P = .001),mutation of TP53 (P < .001), FAB subtypes other than M2 (P= .005), FLT3/ITD (P = .010), high WBC count (more than 100x 10⁹/L) (P = .019), and cytogenetic findings (poor vs others)(P = .024). Multivariate Cox regression analysis with stepwiseselection showed that the mutation of TP53 (odds ratio, 4.002[95% confidence interval (CI), 1.876-8.538]; P < .001), age60 or older (odds ratio, 1.651 [95% CI, 1.131-2.410]; P = .009),and FAB subtypes other than M2 (odds ratio, 1.643 [95% CI, 1.127-2.396];P = .010) were independent poor prognostic factors for overallsurvival (Table 4). When adjusted with age 60 years or older,FLT3/ITD, FAB subtype other than M2, high WBC count (more than100 x 10⁹/L), and mutation of NRAS, mutation of NPM1 was anadverse prognostic factor (odds ratio, 1.949 [95% CI, 1.164-3.268];P = .011). Although careful assessment and further investigationare needed, the mutation of NPM1 may act as a prognostic factorfor overall survival.

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Table 4.. Unfavorable prognostic factors for overall survival in 190 patients, excluding those with the M3 subtype, treated according to JALSG protocols

Because only 1 of 139 patients who achieved CR died during CR,we compared the probability of relapse between patients withand without NPM1 mutations (Figure 2A). Univariate analysisshowed that the unfavorable factors for relapse were mutationof NPM1 (P = .006), FLT3/ITD (P = .007), cytogenetic findings(poor vs others) (P = .007), high WBC count (more than 100 x10⁹/L) (P = .016), FAB subtypes other than M2 (P = .024), andage 60 or older (P = .024). Multivariate Cox regression analysiswith stepwise selection identified that cytogenetic findings(poor vs others) (odds ratio, 3.876 [95% CI, 1.718-8.772]; P= .001) and mutation of NPM1 (odds ratio, 2.106 [95% CI, 1.324-3.350];P = .002) were independent unfavorable factors for relapse (Table 5).

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Table 5.. Unfavorable prognostic factors for relapse in 139 patients with AML, excluding those with the M3 subtype, who achieved CR

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Figure 1.. Mutations in NPM1 exon 12. (A) The mutated nucleotide and the predicted amino acid sequence in NPM1 exon 12 found in the present study are shown in comparison with the wild-type sequence. Type of mutation (mutations A, B, D) is designated according to a previous report. Four novel mutant variants are designated mutations G, H, I, and J. Red and blue indicate nucleotide insertions and termination codons, respectively. Green indicates the conserved residues in mutant NPM. Purple indicates putative residues of a consensus nuclear export signal (Lx[1-3]Vx[2-3]VxL; x indicates any residue). (B) Sequence results after cloning. Boxes indicate inserted 4-bp nucleotides. Arrowhead indicates the position of the insert at nucleotide 960 of the NPM1 gene.

In addition, we analyzed the prognostic value of NPM1 mutationsin 79 patients with normal karyotype. NPM1 mutations were foundin 37 of 79 (46.8%) patients. Of these 79 patients, 59 (74.7%)achieved CR after induction chemotherapy. The CR rate was significantlyhigher in the patients with NPM1 mutations (32 of 37; 86.4%)than in those without (27 of 42; 64.3%) (P = .037 by Fisherexact test). Multivariate logistic regression analysis, includingwild-type NPM1, FAB subtypes (other than M2), presence of FLT3,NRAS, and TP53 mutations, age (older than 60 years), and WBCcount (more than 100 x 10⁹/L) showed that wild-type NPM1 wasthe only independent unfavorable factor for achieving CR (oddsratio, 4.908 [95% CI, 1.011-23.824]; P = .048). Kaplan-Meiercurves according to NPM1 mutation in this group are shown inFigure 2B. Multivariate Cox regression analysis with stepwiseselection showed that age 60 or older was the only poor prognosticfactor for overall survival (odds ratio, 2.068 [95% CI, 1.175-3.641];P = .012). Mutation of NPM1 was not a significant prognosticfactor for overall survival regardless of whatever factors wereused for adjustment by means of Cox analysis. The relapse riskwas analyzed in 59 patients who achieved CR. Multivariate Coxregression analysis with stepwise selection identified thatthe NPM1 mutation was the only independent unfavorable factorfor relapse (odds ratio, 2.096 [95% CI, 1.050-4.186]; P = .036).However, because the patient number of this group was small,larger-scale analysis was required.
FLT3/ITD has been identified as an unfavorable prognostic factorin patients with AML, although the prognostic implications ofFLT3/D835Mt remain unclear. Given that the NPM1 mutation wasassociated with FLT3/ITD, it was important to define the roleof NPM1 mutations alone or in combination with FLT3/ITD forlong-term prognosis. Therefore, we compared the clinical impactof NPM1 mutations in patients with and without FLT3/ITD. Interestingly,mutation of NPM1 was an independent favorable prognostic factorfor CR in patients with FLT3/ITD (odds ratio, 20.8 [95% CI,2.0-200]; P = .011 by multivariate logistic regression analysis),but it did not affect the CR rate in patients without FLT3/ITD.In addition, mutation of NPM1 was a favorable prognostic factorfor overall survival in patients with FLT3/ITD (P = .045), butnot in those without FLT3/ITD. However, mutation of NPM1 wasnot associated with the high relapse rate in patients with FLT3/ITD,whereas it tended to be a worse factor for relapse in thosewithout FLT3/ITD (P = .084) (Figure 3).

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Figure 2.. Kaplan-Meier curves according to NPM1 mutation. (A) Overall survival and relapse risk in all patients. (B) Overall survival and relapse risk in patients with normal karyotype. Statistical difference was evaluated with the log-rank test.

Comparison of mutational status of the NPM1 gene at diagnosis and relapse
Mutational status of the NPM1 and FLT3 genes was compared betweendiagnosis and relapse in 39 AML patients. NRAS and TP53 mutationswere also analyzed in 20 and 29 patients, respectively (Table 6).An NPM1 mutation was found in 17 of 39 patients at diagnosis.Of the 17 patients with NPM1 mutations at diagnosis, 15 carriedthe same mutation at relapse, although 2 patients (unique patientnumber [UPN] 16 and UPN 17) lost the mutation at relapse. InUPN 16, the karyotype of leukemia cells was normal (46XY) atdiagnosis, although it changed to 46XYdel(20)(q1?) at relapse.In contrast, FLT3, NRAS, and TP53 were of the wild type at bothstages. In UPN 17, leukemia cells showed normal karyotype (46XX),FLT3/ITD, and wild-type NRAS and TP53 mutations at diagnosis,and these were retained at relapse.

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Table 6.. Comparisons of mutations between diagnosis and relapse

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Figure 3.. Kaplan-Meier curves according to NPM1 mutation in the FLT3/ITD-positive and -negative patients. (A) In the FLT3/ITD-positive group, the NPM1 mutation was a favorable prognostic factor for overall survival, but did not affect the relapse risk. (B) In the FLT3/ITD-negative group, the NPM1 mutation did not affect overall survival. The NPM1 mutation tended to be a worse factor for relapse in this group, although it was not statistically significant. Statistical difference was evaluated with the log-rank test.

An FLT3 mutation was found in 11 of 39 patients at diagnosis,and all mutations were FLT3/ITD. The FLT3 mutation was lostat relapse in 1 patient, but it emerged at relapse in 4 patientswho did not have the FLT3 mutation at diagnosis. An NRAS mutationwas found in 5 of 20 patients at diagnosis. The NRAS mutationwas lost at relapse in 2 patients, but it emerged at relapsein 1 patient. A TP53 mutation was found in 3 of 28 patientsat diagnosis. The TP53 mutation was lost at relapse in 1 patient,but it emerged at relapse in 1 patient. Taken together, in 11of 39 (28.2%) patients, the gene status of NPM1, FLT3, NRAS,and TP53 was different at diagnosis than it was at relapse (Table 6).However, NPM1 gene status was relatively stable, in contrastto that of FLT3, and was not related to inducing a genotypicchange in leukemia cells at relapse. In addition, age and CRduration were not associated with the genotypic change of leukemiacells at relapse. Importantly, the NPM1 mutation was not associatedwith achieving second CR after first CR.

   Discussion

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

In this study, we found NPM1 mutations in 64 of 257 (24.9%)adult patients with de novo AML. Of the 64 NPM1 mutations, 60were variants reported previously, and 4 were novel. All thenovel variants had a 4-bp insertion at position 960, resultingin the same frameshift as previously reported. The C-terminalof NPM is important to the nuclear localization of NPM,³⁶ andtryptophan residues at positions 288 and 290 are reportedlyassociated with the nucleolar localization of NPM.³⁷ Interestingly,predicted mutant proteins contain a nuclear export signal (NES)motif at the C-terminal, which may be a reason for the cytoplasmicdislocation of mutant NPM.^38,39 All novel variants found inthe present study also contained the NES motif. Therefore, webelieve that the generation of the NES motif by the insertionmutation is strongly associated with the cytoplasmic dislocationof mutant NPM.
FLT3, TP53, and NRAS mutations are the most frequent geneticalterations involved in the pathogenesis of AML. It was reportedthat the NPM1 mutation is closely associated with FLT3/ITD.We found that it is also associated with FLT3/D835Mt, but alarge-scale study is necessary to confirm this association becauseof the small number of patients with FLT3/D835Mt in this study.It is noteworthy that the NPM1 mutation was not associated withTP53, NRAS, and MLL-TD mutations. In fact, the NPM1 mutationwas found in only 2 of 16 patients with the TP53 mutation, althoughthis was not statistically significant. Because the TP53 mutationis known to be present in patients with karyotypic abnormalities,^40,41the NPM1 mutation seems to be infrequent in this group. TheNRAS mutation is negatively related to FLT3/ITD but is foundin all patients with AML, regardless of karyotypic abnormalities.^6,42In contrast, a possible association between MLL-TD and FLT3/ITDwas reported.⁴³ Therefore, to identify factors associated withNPM1 mutations, we performed multivariate logistic regressionanalysis that included the presence or absence of FLT3, TP53,NRAS, and MLL-TD mutations and karyotypic abnormality in 119patients in whom all these genetic alterations were determined.The analysis showed that the normal karyotype (P < .001;odds ratio, 26.0 [95% CI, 6.231-108.73]) and the FLT3 mutation(P < .001; odds ratio, 15.2 [95% CI, 3.690-62.50]) were independentlyassociated with NPM1 mutation. These results suggested thatthe NPM1 mutation might be involved in the pathogenesis of AMLwith and without FLT3 mutations.
The most important finding in the present study is that in patientswith AML, excluding those with the M3 subtype, the NPM1 mutationis a favorable factor for achieving CR after induction chemotherapy,but it implicates a high relapse rate. FLT3/ITD is clinicallydemonstrated to be a poor prognostic factor in patients withAML, especially those in the intermediate-risk group. FLT3/ITDconfers autonomous proliferation to hematopoietic progenitorsthrough its constitutive kinase activity, though alone it isnot sufficient for the development of AML. In the murine APLmodel, the transduction of FLT3/ITD into PML-RARA transgenicbone marrow cells resulted in a shortened latency with increasingpenetration of APL-like disease.⁴⁴ The NPM1 mutation is essentiallyabsent in patients with APL or CBF leukemia, in contrast tothe high frequency of FLT3/ITD and KIT mutations in patientswith APL and CBF leukemia, respectively. Only the mutation ofNPM1 was an independent favorable prognostic factor for achievingCR and a marginally favorable prognostic factor for overallsurvival in patients with FLT3/ITD. However, it did not affectthe CR rate, and its prognostic value for relapse was not significantin patients without FLT3/ITD. Mutant NPM, therefore, might beinvolved in the pathogenesis of AML by its conferring a differentiationblock or properties of self-renewal, or both, to the hematopoieticprogenitors in concert with mutant FLT3, and it might be associatedwith sensitivity to chemotherapy. More recently, it was reportedthat several genes putatively involved in the maintenance ofa stem cell phenotype, such as HOX and JAG1 genes, were up-regulatedin NPMc+ AML cells,⁴⁵ supporting this hypothesis. However, theexact role of mutant NPM in the pathogenesis of AML, especiallywithout FLT3/ITD, has not been fully resolved. Our sequentialanalysis using the paired samples obtained at diagnosis andrelapse demonstrated that the NPM1 mutation is not related toacquiring additional genetic changes in FLT3, TP53, and NRASgenes. In addition, the NPM1 mutation was not a favorable factorfor achieving second CR after relapse, suggesting that unknowngenetic or epigenetic changes might additionally occur in AMLcells with the NPM1 mutation during disease progression. Itis notable that NPM1 mutations were lost at relapse in 2 ofthe 17 patients who had NPM1 mutations at initial diagnosis.Loss of the mutation at relapse has been repeatedly observedin the mutations of FLT3 and NRAS, and these mutations are thoughtof as late or secondary events in leukemogenesis. Loss of theNPM1 mutation at relapse suggests that it is not necessarilyan earlier event and that it is not needed for continuance ofthe disease. However, because NPM is involved in ribosome assembly/transport,cytoplasmic/nuclear trafficking, regulation of DNA polymerasealpha activity, centrosome duplication, acute response of mammaliancells to environmental stress, and stabilization of the p53pathway,^25,26,46-48 it is possible that mutant NPM also hasa multifunctional role in the pathogenesis of AML. Alternatively,mutant NPM might use its multiple functions according to thegenetic state of leukemia progenitors. Further biologic studiesare necessary to clarify how mutant NPM is involved in the pathogenesisof AML and what kinds of genetic or epigenetic alterations cooperatewith mutant NPM for the development of AML.

   Acknowledgements

This study was performed in cooperation with JALSG. We thankManami Kira for secretarial assistance.

   Footnotes

Submitted April 28, 2005; accepted June 12, 2005.
Prepublished online as Blood First Edition Paper, June 30, 2005;DOI 10.1182/blood-2005-04-1733.

Supported by Grants-in-Aid from the Ministry of Health, Labor,and Welfare and from the Scientific Research and the 21st CenturyCOE Program "Integrated Molecular Medicine for Neuronal andNeoplastic Disorders" of the Ministry of Education, Culture,Sports, Science, and Technology, Japan.

T.S., H.K., R.U., and T.N. designed the research protocol; T.S.,H.K., K.O., A. Tomita, and S.Y. performed the genetic analysis;T.S., H.K., R.S., and T.N. analyzed the data; H.K., K.O., R.S.,Y.K., S.M., N.A., K.K., F.Y., C.S., H.A., M.N., T.M., K.S.,A. Takeshita, R.U., T.K., N.E., and T.N. collected samples andmanaged clinical data; and T.S., H.K., and T.N. wrote the paper.

The online version of this article contains a data supplement.

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 U.S.C. section 1734.

Reprints: Hitoshi Kiyoi, Department of Infectious Diseases, Nagoya University School of Medicine, 65 Tsurumai-cho, Showa-ku, Nagoya 466-8560, Japan; e-mail: kiyoi{at}med.nagoya-u.ac.jp.

   References

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

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  Copyright © 2005 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2005 by American Society of Hematology Online ISSN: 1528-0020