Global approach to the diagnosis of leukemia using gene expression profiling

doi:10.1182/blood-2004-12-4938

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Blood, 15 August 2005, Vol. 106, No. 4, pp. 1189-1198.
Prepublished online as a Blood First Edition Paper on May 5, 2005; DOI 10.1182/blood-2004-12-4938.

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CLINICAL OBSERVATIONS, INTERVENTIONS, AND THERAPEUTIC TRIALS
Global approach to the diagnosis of leukemia using gene expression profiling
Torsten Haferlach, Alexander Kohlmann, Susanne Schnittger, Martin Dugas, Wolfgang Hiddemann, Wolfgang Kern, and Claudia Schoch
From the Laboratory for Leukemia Diagnostics, Department of Internal Medicine III, University Hospital Grosshadern, Ludwig-Maximilians-University, Munich, Germany; and the Department of Medical Informatics, Biometrics and Epidemiology, Ludwig-Maximilians-University, Munich, Germany.

   Abstract

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Accurate diagnosis and classification of leukemias are the basesfor the appropriate management of patients. The diagnostic accuracyand efficiency of present methods may be improved by the useof microarrays for gene expression profiling. We analyzed geneexpression profiles in 937 bone marrow and peripheral bloodsamples from 892 patients with all clinically relevant leukemiasubtypes and from 45 nonleukemic controls by U133A and U133BGeneChip arrays. For each subgroup, differentially expressedgenes were calculated. Class prediction was performed usingsupport vector machines. Prediction accuracy was estimated by10-fold cross-validation and was assessed for robustness ina 100-fold resampling approach using randomly chosen test setsconsisting of one third of the samples. Applying the top 100genes of each subgroup, an overall prediction accuracy of 95.1%was achieved that was confirmed by resampling (median, 93.8%;95% confidence interval, 91.4%-95.8%). In particular, acutemyeloid leukemia (AML) with t(15;17), AML with t(8;21), AMLwith inv(16), chronic lymphatic leukemia (CLL), and pro–B-cellacute lymphoblastic leukemia (pro–B-ALL) with t(11q23)were classified with 100% sensitivity and 100% specificity.Accordingly, cluster analysis completely separated all 13 subgroupsanalyzed. Gene expression profiling can predict all clinicallyrelevant subentities of leukemia with high accuracy.

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

The diagnosis and classification of leukemia rely on the simultaneousapplication of multiple techniques. Cytomorphology and histomorphologyare combined with cytochemistry and multiparameter flow cytometryto assign the diagnostic sample to the correct entity. Furthermore,chromosomal analysis, often supplemented by fluorescence insitu hybridization (FISH), and molecular techniques, such aspolymerase chain reaction (PCR), is needed to definitively confirmthe diagnosis. A comprehensive and standardized algorithm fora diagnostic workflow and an effective and carefully designedcombination of methods is essential to guarantee that all therequired diagnostic information is gathered.
This huge amount of laboratory assessment is necessary not onlyto diagnose and classify leukemia samples correctly but to detectbiologically homogeneous entities that require specific treatmentapproaches. Thus, the detailed leukemia classification proposedby the French-American-British (FAB)^1,2 Cooperative Group hasbeen improved by thoroughly defined genetic and other characteristics,resulting in the new World Health Organization (WHO) classification.³This also led to new prognostic markers and even to disease-specifictherapeutic approaches. The prime example for this strong linkbetween a comprehensive diagnosis and a disease-specific treatmentapproach has been the use of all-trans retinoic acid (ATRA)in patients with acute promyelocytic leukemia. Both the correctdiagnosis and the efficacy of the specific treatment are basedon the presence of the translocation (15;17) and of the correspondingPML/RARA fusion gene.^4-6 Although it did not result in the developmentof a new targeted drug therapy, identifying acute myeloid leukemia(AML) with a complex aberrant karyotype, depending on the ageof the patient, is nonetheless highly relevant for the managementof the patient. This dismal diagnosis—again, dependingon the age of the patient—is the basis for the decisionto perform allogeneic stem cell transplantation very early oreven to withhold antileukemia therapy.^7-10 The recent introductionof imatinib mesylate into the therapeutic management of patientswith chronic myeloid leukemia (CML) has revolutionized the treatmentstrategies for this disease and may change therapeutic conceptsfor BCR/ABL-positive acute lymphoblastic leukemia (ALL) in thenear future.^11-16 Again, the basis for the correct diagnosisand the specifically targeted therapy is the presence of thegenetic alteration, the t(9;22) translocation. In addition,the BCR/ABL fusion gene is increasingly used to sensitivelyassess response to therapy by monitoring minimal residual disease(MRD) levels.¹⁷ In patients with acute leukemias and chroniclymphatic leukemia (CLL), monitoring of MRD is increasinglyused to guide risk-adapted therapy.^18-22
To achieve the correct and complete diagnosis in each analyzedsample, a modern, state-of-the-art laboratory must provide significantresources for laboratory equipment, working time, and skilled,experienced personnel. What is needed is a novel diagnostictool that provides the opportunity to satisfy diagnostic needswhile enabling efficient use of resources.
Microarray analysis used to perform gene expression profilingmay be the method of choice in this regard^23-25 because it allowssimultaneous detection of the expression of nearly all humangenes in one experimental approach, thereby providing maximalinsight into gene regulation and gene alterations in the analyzedsample on the transcriptional level. Although many studies exploitedthis technique to gain clues to the pathogenesis of a largevariety of malignant diseases and to characterize unidentifieddisease subentities, little focus has been applied to gene expressionprofiling for diagnostic purposes.^26-28
Here, we describe the results of an extensive microarray studyon leukemia samples that was performed in parallel with allstandard techniques and that resulted in a global, one-step,diagnostic approach. In 937 samples from patients with newlydiagnosed leukemia and from nonleukemic controls, we focusedon all leukemic subentities clinically relevant with respectto specific treatment approaches and prognostication. Usingunsupervised and supervised biostatistical methods based primarilyon support vector machines (SVMs), we confirmed and reproduced12 predefined leukemia subtypes and separated all from eachother and from nonleukemic control bone marrow samples withan accuracy of 95.1%. Thus, the single method, gene expressionprofiling using microarrays, may effectively be applied as acomplementary diagnostic method in patients with leukemia andmay even substitute for other methods in the future.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patient and control samples
Nine hundred thirty-seven bone marrow and peripheral blood samplesfrom patients with newly diagnosed leukemia and from nonleukemiccontrols were included in the present analysis. CLL samplesconsisted of peripheral blood, whereas samples from all otherentities in general consisted of bone marrow. Samples were sentto the Laboratory for Leukemia Diagnostics in Munich, Germany,between February 1998 and February 2004 for reference diagnosisfrom local and national hospitals. The median shipment timewas 1 day (range, 0-3 days). All samples underwent standardizedprocessing, including sample central registration,²⁹ preparation,and evaluation by cytomorphology,³⁰ cytochemistry, multiparameterimmunophenotyping,³¹ cytogenetics,³² fluorescence in situ hybridization(FISH), and molecular genetics.³³ Stabilized cell lysates werestored at –80°C for a median of 13 months (range,0-67 months). Diagnoses and other sample and patient characteristicsare given in Tables 1 and 2. After 800 samples had been identifiedfor inclusion in the study, another 137 samples were selectedaccording to diagnosis to achieve a distribution among the diseasesubtypes, thereby ensuring an adequately powered study. In allsamples with balanced translocations, the corresponding fusiontranscript was verified on the molecular level—that is,PML/RARA for t(15;17), AML1/ETO for t(8;21), CBFB/MYH11 forinv(16) or t(16;16), MLL/and various partner genes for t(11q23)in AML and ALL, and BCR/ABL for t(9;22) in ALL and CML. In addition,in each of these samples and for MYC/IGH for t(8;14), FISH wasapplied using standard procedures.³⁴

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Table 1.. Sample and patient characteristics

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Table 2.. Distribution of leukemia subtypes

Before therapy, all patients gave their informed consent forparticipation after having been advised of the purpose and investigationalnature of the study and of the potential risks. The study designadhered to the tenets of the Declaration of Helsinki and wasapproved by the ethics committees of the participating institutionsbefore its initiation.
Leukemia entities selected for identification by gene expression profiling
The focus of the present study was to identify all leukemiasubgroups that were clinically relevant with regard to specifictreatment and prognostication. Along with the distinctions amongthe 4 main categories of leukemia (AML, ALL, CML, CLL), theserelevant groups also comprised specifically defined subentities.In addition to the group designated "nonleukemia"—thosewith healthy bone marrow (n = 11), elevated white blood cell(WBC) counts during infection (n = 8), slightly elevated WBCcounts of unknown origin (n = 6), staging non-Hodgkin lymphomawithout bone marrow involvement (n = 4), staging Hodgkin diseasewithout bone marrow involvement (n = 3), staging cutaneous mastocytosiswithout bone marrow involvement (n = 3), drug-induced bone marrowfailure in early regeneration (n = 3), liver cirrhosis (n =2), iron deficiency (n = 2), osteoporosis (n = 1), vitamin B12deficiency (n = 1), or idiopathic thrombocytopenic purpura (n= 1)—the following 12 clinically relevant subgroups wereanalyzed: AML with t(15;17), AML with t(8;21), AML with inv(16),AML with normal karyotype or so-called "other" cytogenetic abnormalities,AML with 11q23/MLL rearrangement, AML with complex aberrantkaryotype, pro–B-ALL with t(11q23), mature B-ALL witht(8;14), c-ALL/pre–B-ALL with or without t(9;22), T-cellALL (T-ALL), CML, and CLL.
Gene expression profiling, data analysis, and real-time PCR
Additional information on methods with regard to gene expressionprofiling, data analysis, and real-time PCR are given in SupplementalDocument S1 (see the Supplemental Materials link at the topof the online article, at the Blood website).

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Prediction of 13 subgroups
Predicting the respective leukemia type or subtype based ondifferential gene expression signatures was approached usingSVMs. The complete data set was randomly, but equally, splitinto training and independent test cohorts for the 13 subgroups.Then differentially expressed genes were identified in the trainingset calculated by means of t test statistic, and an SVM modelwas built based on the genes that demonstrated differentialexpression among the respective subclasses in the training set.
This SVM model was used to predict samples in the test cohort.Application of the top 100 genes per group resulted in the bestprediction accuracy (superior to top 20, 50, 150, 200, 250,and 300 genes, respectively; data not shown) and were used forall subsequent analyses (for a description of the genes, seethe supplemental material). Table 3 represents a confusion matrixof subgroup predictions based on their gene expression signaturesusing a 10-fold cross-validation approach (9 of 10 for trainingand 1 of 10 for testing, with 10 iterations so that each sampleis classified once). Overall, a 95.1% accuracy of subgroup predictionwas achieved analyzing 13 subgroups. Specifically, the highestaccuracy was achieved for 7 of the 13 subgroups—AML witht(15;17), 100% accurate predictions; AML with inv(16), 98%;CLL, 97.8%; CML, 97.3%; AML normal/other, 97.3%; pro–B-ALLwith t(11q23), 96.2%; and AML with t(8;21), 94.7%. The presenceof a cryptic rearrangement (inv(16), n = 1; t(16;16), n = 3;AML with t(11q23)/MLL, n = 1; ALL with t(9;22), n = 2; CML witht(9;22), n = 2; and CML with variant t(9;22), n = 3)³⁵ had noimpact on the accuracy of classification. These patients, therefore,were grouped together with patients carrying the respectiveovert cytogenetic abnormality. For the other 6 subgroups, thepercentages of accurate predictions ranged between 83.3% and93.3%.

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Table 3.. Prediction confusion matrix for 13 subtypes determined by 10-fold cross-validation

Most of the misclassifications occurred in subgroups that eitherhad relatively low sample numbers or were characterized by highintra-subgroup biologic heterogeneity. The first aspect clearlyapplies to mature B-ALL with t(8;14) with a sample number of12 and 83.3% accurate predictions. The latter aspect is reflectedin AML with t(11q23) (89.4% accurate predictions) with balancedtranslocations involving the MLL gene and 6 different fusionpartner genes (AF4, AF6, AF9, AF10, ELL, ENL). Another exampleof biologic heterogeneity is AML with complex aberrant karyotype(88% accurate predictions) composed of a wide range of 3 to30 chromosomal abnormalities (median, 9). As anticipated, mostof the misclassifications of these groups (4 of 5 for AML witht(11q23) and 8 of 9 for AML with complex aberrant karyotype)were attributed to a prediction of the samples as AML normal/other.A third aspect to consider is the relative similarity of distinctsubgroups with regard to specific characteristics, such as flowcytometrically detected expression of myeloid antigens on immatureT-ALL samples.³⁶ Probably because of these complexities, 4 of32 patients with T-ALL in the present series were classifiedas having AML normal/other. Importantly, the inclusion of "AMLnormal" and "AML other" into the analyses as 2 separate groupsdid not result in superior classification accuracy (SupplementalTables S3-S6).
To assess the robustness of class prediction, a resampling approachwas applied, which is to say the complete SVM classificationprocedure was repeated 100 times. For each of the 100 runs,all samples were randomly divided into a training set (two thirdsof all samples; n = 625) and a test set (one third of all samples;n = 312). Thus, the test set for each run consisted of c-ALL/pre–B-ALL(n = 28), pro–B-ALL with t(11q23) (n = 9), mature B-ALLwith t(8;14) (n = 4), T-ALL (n = 10), AML with t(15;17) (n =14), AML with t(8;21) (n = 12), AML with inv(16) (n = 16), AMLwith t(11q23) (n = 16), AML with complex karyotype (n = 25),AML with normal karyotype or other aberrations (n = 123), CLL(n = 15), CML (n = 25), and nonleukemia samples (n = 15). Thematrix in Table 4 gives the average number of class predictionsas determined after 100 runs of SVM-based classifications. Forexample, 9 pro–B-ALL with t(11q23) samples were predictedby the algorithm 900 times (each sample 100 times). Of the 900predictions, the class label pro–B-ALL with t(11q23) wasassigned correctly 854 times (ie, on average 8.54 per run).In 2 individual predictions, pro–B-ALL with t(11q23) sampleswere predicted as c-ALL/pre–B-ALL, and in 44 predictionsthey were predicted as AML with normal karyotype or other aberrations.

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Table 4.. Prediction confusion matrix for 13 subtypes as determined by resampling using SVM

Confirming the data obtained by 10-fold cross-validation, theoverall median accuracy amounts to 93.8% (95% CI, 91.4%-95.8%).In particular, and similar to the 10-fold cross-validation approach,a very high degree of accurate predictions was achieved in 7of the 13 subgroups: AML with t(15;17), 100% median accuracy;AML with inv(16), 98.1%; CLL, 97.5%; CML, 95.3%; AML normal/other,96.8%; pro–B-ALL with t(11q23), 94.9%; and AML with t(8;21),95.3%. For the other 6 subgroups, the median prediction accuracyrates ranged between 64.3% and 92.3%. Thus, the results obtainedfor the subgroups by applying the resampling approach are highlyconsistent with those obtained by 10-fold cross-validation andstrongly confirm the capability of gene expression profilingto predict leukemia subtypes. The reasons for the misclassificationsare most likely the same as those described, in particular therelatively low sample number of patients with mature B-ALL witht(8;14).
Sensitivities and specificities of the predictions for eachof the 13 subclasses are given in Table 5. According to theaccuracy data given, the specificity overall is very high—morethan 99% for all but one subgroup. Because most misclassifiedsamples were classified as AML normal/other, the specificityof this subgroup was slightly lower than it was for other subgroupsand amounted to 93.65%. The median sensitivity ranged between75% and 100% for all subgroups because of the reasons discussedfor the results of the 10-fold cross-validation.

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Table 5.. Sensitivity and specificity for leukemia classification using SVM in 13 subgroups

Cluster analysis of 13 subgroups
To further validate the findings described, supervised clusteranalyses (CAs) and principal component analyses (PCAs) usingthe top 100 differentially expressed genes for each subgroupwere performed for the 13 groups analyzed and for the pairedcomparison of selected groups. CAs of all of the analyzed samplesreflect the clearly differing gene expression patterns of the13 groups, resulting in a highly accurate separation of thislarge and comprehensive series of 937 samples (Figure 1). Applying3-dimensional PCA (Figure 2), the power of the gene expressionprofile–based leukemia classification is demonstratedby the clear separation of T-precursor ALL from c-ALL/pre–B-ALL(with or without t(9;22)/BCR/ABL). Similarly, 3-dimensionalPCAs provide a clear distinction between both t(9;22)–positiveentities, CML and c-ALL/pre–B-ALL (Figure 3). Interestingly,the one sample of t(9;22)–positive c-ALL/pre–B-ALLshown in proximity to the CML samples carries the BCR-ABL typeM-bcr (p210), which is more frequently present in CML than inALL. Furthermore, this sample is characterized by only 50% leukemicbone marrow infiltration; thus, the normal hematopoiesis presentin this sample, which is largely myelomonocytic, and the forcedassignment to either of the 2 groups are the likely reasonsfor this result.

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Figure 1.. Hierarchical cluster analysis of 937 samples. Analysis of 937 samples (columns) using a set of 1019 differentially expressed genes (rows). The normalized expression value for each gene is coded by color (SD from mean). Red cells indicate high expression, and green cells indicate low expression. Bars separate the major leukemia types. For each of the 13 classes, the top 100 differentially expressed genes, according to t test statistic, were used. Of the 1300 genes, 281 were repeatedly identified as important diagnostic markers and overlapped among the lists of the top 100 genes, resulting in 1019 nonoverlapping genes.

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Figure 2.. Distinction between precursor B-ALL and T-ALL. In 3-dimensional PCA, 114 ALL samples were projected into the feature space consisting of a combination of the top 100 differentially expressed genes when comparing precursor B-ALL with the other 12 classes or T-ALL with the other 12 classes. Data points with similar characteristics will cluster together. Here, a single color-coded sphere represents each patient's expression pattern. The respective label (ie, precursor B-ALL or T-ALL) was unknown to the algorithm. Labels and coloring of the classes were added after the analysis of means for better visualization. Pre–B-ALL samples (n = 82) are blue and include 42 c-ALL/pre–B-ALL with t(9;22) and 40 c-ALL/pre–B-ALL without t(9;22). T-ALL samples (n = 32) are turquoise.

Identification of cortical T-ALL and pre–B-ALL with t(9;22)
To further define the classification capabilities of our approach,we aimed at identifying the clinically distinct entities, c-ALL/pre–B-ALLwith t(9;22) and cortical T-ALL, from among the groups classifiedas c-ALL/pre–B-ALL and T-ALL, respectively.
With regard to c-ALL/pre–B-ALL, cluster analysis (Figure 4)showed that most (61 of 82; 74%) of the patients had c-ALL/pre–B-ALLwithout t(9;22) or with t(9;22). The remaining 21 (26%) patientshad a third branch characterized by a gene expression profileclearly different from that of the other 2 groups. Accordingly,the 10-fold cross-validation analysis (allowing separation into2 groups only) revealed an accuracy of 82.9%. Misclassificationsoccurred in both directions. Patients with t(9;22) were classifiedas without it and vice versa. Resampling of the training andtest sets, respectively, applying 100 runs of SVM-based classification(median accuracy, 77.8%; range, 61%-90.8%) indicated that thesemisclassifications were not limited to distinct samples. Percentagesof misclassifications per sample ranged from 3.1% to 88.1%,probably reflecting a significant overlap of gene expressionsignatures between both groups or resulting from the presenceof a clinically unidentified third group of c-ALL/pre–B-ALL.

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Figure 3.. Distinction between c-ALL/pre–B-ALL with t(9;22) and CML. In 3-dimensional PCA, 117 samples were projected into the feature space consisting of a combination of the top 100 differentially expressed genes when comparing c-ALL/pre–B-ALL with t(9;22) samples with the other 12 classes and CML with the other 12 classes. Data points with similar characteristics will cluster together. A single color-coded sphere represents each patient's expression pattern. The respective label (pre–B-ALL or CML) was unknown to the algorithm. Labels and coloring of the classes were added after the analysis of means for better visualization. c-ALL/pre–B-ALL with t(9;22) samples (n = 42) are red, and CML samples (n = 75) are green.

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Figure 4.. Identification of c-ALL/pre–B-ALL samples with or without t(9;22). Analysis of 82 c-ALL/pre–B-ALL samples based on a supervised identification of differentially expressed genes among 42 patients demonstrating a t(9;22)/BCR-ABL and 40 patients without t(9;22). The labels and coloring of the classes were added after the analysis of means for better visualization. (A) In the hierarchical cluster analysis, the normalized expression value for each gene (given in rows) is coded by color (SD from mean). Red cells indicate high expression, and green cells indicate low expression. Most (61 of 82; 74%) patients were in the branch of c-ALL/pre–B-ALL without t(9;22) (left branch) or in the branch of c-ALL/pre–B-ALL with t(9;22) (right branch). The remaining 21 (26%) patients were in a third branch characterized by a gene expression profile clearly different from the 2 other groups (middle branch). (B) In 3-dimensional PCA, the c-ALL/pre–B-ALL samples were projected into the feature space consisting of the top 100 differentially expressed genes when comparing t(9;22)–positive (red) with t(9;22)–negative (purple) patients. Data points with similar characteristics cluster together. A single color-coded sphere represents each patient's expression pattern.

With regard to patients with T-ALL, the separation of corticalT-ALL samples from immature T-ALL samples is clear, as shownin the cluster analysis (Figure 5). Interestingly, 2 samplesof immature T-ALL show a gene expression profile slightly differentfrom that of the other immature T-ALL samples, as visualizedby cluster analysis (Figure 5). By standard diagnostics, these2 samples indicated pre–T-ALL without any specific featurefor cortical T-ALL. They are negative for CD1a in immunophenotypingand show no specific cytogenetic abnormality: 46,XX and 46,XX,t(8;14)(q24;q11),+10, t(11;14)(p12;q11). In fact, these 2 samplesare those lying nearest to the cortical T-ALL samples in thePCA. According to the relative vicinity of these 2 samples tosamples of cortical T-ALL, the accuracy of the 10-fold cross-validationis 84.38%, and resampling applying 100 runs of SVM-based classificationresults in a median accuracy of 80% (range, 60%-100%).
The separation of samples with AML and normal karyotypes fromthose with AML and "other" cytogenetic aberrations was not approachedin the present study because the prognosis for each subgroupwas identical when applying a standardized treatment approach^30,37,38(Figure S1). We intended to approach the data from a clinicalpoint of view, but there was no clear-cut relevance for thedistinction between these 2 groups. Additional data with regardto technical aspects of sample target preparation, scan quality,and validation of significant genes by real-time PCR are givenin the supplemental material (Supplemental Figure S2).

   Discussion

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Diagnosing and classifying leukemias is clinically a highlyrelevant task that requires a comprehensive and well-structuredapproach in the laboratory to guarantee the appropriatenessof the results. Significant resources with regard to time, well-trainedand skilled personnel, and laboratory space and equipment areneeded to cover this approach. Furthermore, the interlaboratoryreproducibility of currently applied diagnostic methods (cytomorphology,cytochemistry, immunophenotyping, cytogenetics, and moleculargenetics) ranges between only 56% and 90% in experienced hands;clearly, then, improvement is needed.^9,39-43 Gene expressionprofiling using microarray technology may optimize leukemiadiagnostics and overcome the shortcomings of current methods.

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Figure 5.. Distinction between immature and cortical T-ALL samples. Analysis of 32 T-ALL samples based on a supervised identification of differentially expressed genes between 12 immature T-ALL samples and 20 cortical T-ALL samples. Labels and coloring of the classes were added after analysis for better visualization. (A) In hierarchical cluster analysis, the normalized expression value for each gene (given in rows) is coded by color (SD from mean). Red cells indicate high expression, and green cells indicate low expression. (B) In 3-dimensional PCA, T-ALL samples were projected into the feature space consisting of the top 100 differentially expressed genes when comparing patients with immature (orange) and cortical (purple) T-ALL. Data points with similar characteristics cluster together. A single color-coded sphere represents each patient's expression pattern.

The present study focused on the identification of all clinicallyrelevant subtypes of leukemia by gene expression profiling andfound significant differences for intragroup separation withinthe 4 main leukemia groups (AML, ALL, CML, and CLL). With regardto AML, more than 50 recurrent cytogenetic abnormalities havebeen described. However, reliable data about their prognosticimpact are available for only the most frequent ones. Theseinclude t(15;17), t(8;21), and inv(16), which are associatedwith a favorable outcome, and complex aberrant karyotypes andt(11q23), which are associated with an unfavorable outcome.^8-10,32,44The remaining abnormalities, normal karyotypes, and so-calledother cytogenetic abnormalities, are associated with an intermediateprognosis. Supplemental Figure S1 demonstrates that the separationbetween these subgroups results in highly different prognoses,supporting the clinical relevance of the selection of AML subgroupsin the present study. The same applies for the cohort selectedfor the present microarray analysis. In addition, the age distributionof the analyzed cohort is similar to the true age distributionof patients with AML and the other diseases analyzed. With regardto clinical relevance, similar characteristics applied to thedifferent entities of ALL. Besides the separation of T-precursorALL from B-precursor ALL, clinically relevant because of differenttreatment strategies, it is important to identify patients withpro–B-ALL and t(11q23) c-ALL or pre–B-ALL and t(9;22)and with mature B-ALL and t(8;14). These subentities differhighly with respect to prognostic impact and require substantiallydifferent therapies, which is true for mature B-ALL in particular.^11,45The overall smaller numbers of participants with CLL, CML, andnonleukemia were chosen because these entities are biologicallyand clinically more homogeneous than the acute leukemia casesdiscussed.
The present study demonstrates a very high degree of accuracyfor the correct assignment of bone marrow samples to all clinicallyrelevant subgroups of leukemia and to normal bone marrow, respectively.An essential basis for the achievement of this accuracy wasthe careful and comprehensive use of standard methods to characterizeall the samples before they were subjected to microarray analysis.In addition to the use of cytomorphology and cytochemistry,the samples were processed through immunophenotyping, cytogenetics,and molecular genetics to allow the identification of subtype-specificgene expression patterns and to exclude any misclassificationof samples or overlaps among the subcategories in the microarrayanalyses.
Six different AML subgroups were detected in the present study.For the classification of AML with t(15;17), t(8;21), and inv(16),the highest degree of accuracy was achieved, respectively, with42 of 42, 36 of 38, and 48 of 49 correct assignments by 10-foldcross-validation and an average number of correct predictionsof 14 of 14, 11.43 of 12, and 15.7 of 16, respectively, by resampling.Accordingly, all the median sensitivities and specificitieswere 100%. This is in line with previous reports describinga unique biologic background for these subentities,^46-48 whichis reflected in distinct gene expression profiles.^49-52 However,because the latter have not yet been assessed by microarrayanalysis in the context of the full spectrum of AML and theother leukemias, the present study adds important informationby clearly demonstrating that, based on their distinct features,these subentities can be accurately predicted even in the contextof the heterogeneous background of other leukemias. The other3 AML subgroups—AML with t(11q23)/MLL, AML with complexkaryotype, and AML normal/other—are biologically moreheterogeneous, as reflected by different partner genes of theMLL gene and overall heterogeneity with regard to cytogeneticand molecular genetic aberrations. With these complexities inmind, it was anticipated that misclassifications would occur.Of the 24 misclassifications (total, 491 classifications) inthese subgroups during 10-fold cross-validation, only 4 weremisclassifications into the non-AML subgroups. As a consequence,though the median specificities for AML with t(11q23) and forAML with complex aberrant karyotypes were very high (99.66%and 99.65%, respectively), the median specificity for AML normal/otherof 93.65% points to the need for further improvement in theapplied method or for the use of supplemental analyses, particularlybecause a small number of patients with ALL (n = 11), CLL (n= 1), CML (n = 2), and nonleukemia (n = 2) were classified intothis subgroup by 10-fold cross-validation.
With the exception of these 3 samples, there were no misclassificationsin CLL and CML by 10-fold cross-validation. Accordingly, therewere 14.62 of 15 and 23.82 of 25 correct assignments, respectively,by resampling in these entities. As a result, the median sensitivities(100% and 96%) and the clinically most important median specificities(100% and 99.65%) were very high for these distinct diseaseentities.
All 4 subgroups of ALL analyzed in the present study could beclassified with a high median accuracy (99.65% for c-ALL/pre–B-ALL;100% for the other subgroups). As discussed, most (11 of 13)misclassifications occurred in the AML normal/other group. Interestingly,these samples did not feature the immunophenotype of an aberrantexpression of myeloid antigens, which is often observed in patientswith ALL.
Given that previous studies reported on the difficulties indistinguishing c-ALL/pre–B-ALL with t(9;22) from othertypes of B-precursor ALL, resulting in a prediction accuracyrate of 80%,²⁶ the approach in the present study was to includepatients with c-ALL/pre–B-ALL combined as one subgroup,irrespective of the presence of t(9;22), in the analysis andto separate patients positive for t(9;22) from those withoutit. Although the separation of c-ALL/pre–B-ALL from theother entities has been straightforward, we also observed difficultiesin separating t(9;22)–positive patients from t(9;22)–negativepatients and achieved only 82.9% accuracy. Interestingly, clusteranalysis demonstrated that most patients were accurately classifiedin 1 of the 2 categories; however, a third branch became evident,revealing a gene expression pattern distinct from that of theother 2 groups. The hypothesis that a further and not yet identifiedgenetic lesion could be responsible for this third branch hasbeen discarded because cluster analysis and SVM did not reveala reproducible gene expression pattern different from that ofthe other 2 groups (data not shown). Furthermore, the use ofSVM with differentially expressed genes selected based on thecomparison of only the first 2 more homogeneous groups did notresult in a more accurate assignment of samples of the thirdgroup either (data not shown). Taken together, these pointssupport the concept that BCR/ABL represents a type 1 mutation⁵³and that downstream pathways are shared by many other mastergenes. Thus, the gene expression profile of patients with BCR/ABL-positiveALL is not highly reproducible (Figure 4), and future microarray-baseddiagnostic tools should include oligonucleotides targeting thebcr/abl fusion transcript to accurately predict BCR/ABL-positiveALL with greater accuracy. It is anticipated this would increasethe sensitivities and specificities for the classification ofthe other subgroups.
Another clinically relevant subgroup has been approached ina second step. After T-ALL was distinguished from all otherentities, immature T-ALL was distinguished from cortical T-ALL,which, in the clinical setting, is characterized by a favorableprognosis.³⁶ Again, the separation of both entities has beenhighly accurate, with the exception of 2 samples that originallywere classified by immunophenotyping as immature T-ALL. It isimportant to note that the definition of cortical T-ALL in thiscontext is based only on positivity for CD1a,⁵⁴ whereas otherT-cell markers, such as CD7, CD2, CD5, CD4, and CD8, may bepositive in either subgroup. Intriguingly, though the use ofCD1a is a diagnostic standard, the present analysis suggeststhat in the 2 misclassified patients, the overall gene expressionprofile is similar to that of the cortical T-ALL signature.Thus, these 2 patients may have cortical T-ALL featuring anaberrant lack of CD1a expression rather than truly immatureT-ALL. As a consequence of our studies, the classification ofcortical T-ALL may be based not only on positivity for CD1abut also on other markers, such as PAWR.⁵⁵
Further implications may be gained from analyzing the cellularfunction of differentially expressed genes. It is known thatdexamethasone leads to the down-regulation of CARD4,⁵⁶ whichencodes a proapoptotically acting protein.^57,58 Because CARD4is highly expressed in cortical T-ALL, corticoid therapy maybe less effective in this entity than in immature T-ALL. However,clinical studies are needed to prove this hypothesis.
A particularly important issue that has not yet been substantiallyaddressed in other microarray studies^59-61 is the identificationof nonleukemic bone marrow and its distinction from all leukemiasubtypes. In the present study, 42 of 45 nonleukemia sampleshave been predicted accurately, whereas 1 sample was classifiedas AML with t(11q23) and 2 samples were classified as AML normal/otherby 10-fold cross-validation. Accordingly, the median accuracyapplying resampling is 13.2 of 15. Importantly, the median specificityfor nonleukemia is 99.7%, and the sensitivity is 90%. Thus,until improvements of the applied methods are achieved thatbetter characterize the heterogeneous subgroup of AML normal/other,it seems appropriate to add conventional methods if the microarrayanalysis result assigns a sample to the latter subgroup. Incontrast, because of its high specificity, the nonleukemia classificationcan be the basis to exclude the presence of leukemia in a givensample analyzed.
In general, there are 2 strategies to handle the occurrenceof misclassifications obtained by microarray analysis. The firstis to identify the most frequent false-positive result—thesubgroup with the lowest specificity—and to add conventionaldiagnostics to confirm or revise a diagnosis of malignancy.Clearly, this applies for AML normal/other with a median specificityof 93.7% (95% CI, 90.2%-96.6%). Through the use of cytochemistry,immunophenotyping, and cytogenetics, distinguishing this subgroupfrom c-ALL/pre–B-ALL, AML with t(11q23), and AML withcomplex aberrant karyotype is straightforward though resourceconsuming. Another possible application for additional methodsis the use of PCR to identify or exclude the presence of theBCR/ABL fusion gene once c-ALL/pre–B-ALL is diagnosed.
The second and more promising strategy would be an improvementin the capabilities of microarray technology by taking advantageof the additional representation of fusion gene–specificoligonucleotides. By this approach, many of the misclassificationsshould be avoidable; for example, c-ALL/pre–B-ALL witht(9;22) should be identifiable by the detection of BCR/ABL,as should AML with t(11q23) by the detection of fusion genesinvolving MLL and various partners.⁶² Following this approachwould potentially result in even higher rates of accuracy inthe subgroups discussed and in improving accuracy in the othersubgroups.
Even more subgroups, particularly of AML, have been suggestedto feature a homogeneous biologic background with potentialimpact on the clinical course of patients affected by theseentities.⁶³ Examples are mutations of CEBPA,⁶⁴ length mutationsof FLT3,³³ and partial tandem duplications of MLL.⁶⁵ However,because this evidence is still under evaluation in clinicaltrials, these subgroups are not within the focus of the presentstudy.
A growing body of published microarray studies address the identificationof specific gene-expression profiles in distinct subentitiesof leukemia. Along this line, the respective groups of AML withrecurrent balanced translocations and of AML with trisomy 8have been described to carry a typical genetic signature, which,in some cases, is highly specific.^28,50,66,67 The present analysisfollowed these important studies and provided the opportunity,by focusing on all clinically relevant subtypes of chronic andacute leukemias in a single comprehensive approach, to buildon these signatures for a highly accurate diagnostic tool capableof predicting leukemia subtypes. In addition, the separationof leukemia samples from samples with nonmalignant diseasesand healthy samples has been accomplished. In accordance withthese analyses of leukemia, it is anticipated that similar approachescan be taken to diagnose and classify myelodysplastic syndromesand lymphomas.^61,68,69
One possible result of this study could be the widespread useof microarray technology entailing a carefully designed, comprehensiveapproach to the diagnosis of leukemia and representing a significantimprovement over current diagnostic procedures through greateraccuracy and efficiency. Thus, the 1-day (cytomorphology, immunophenotyping)to 1-week (metaphase cytogenetics) turn-around time for currentprocedures may be reduced to 1 to 2 days, or even less, withmicroarray protocols. This technology should also provide significantinsight into the specific genetic alterations of distinct entities,allowing the detection of novel markers that can be targetedby PCR-based methods and multiparameter flow cytometry to quantifyMRD during the course of antileukemia treatment.⁷⁰ Identifyingprognostic markers or marker constellations that will predictthe response to antileukemia treatment is another clinicallyrelevant topic and will be covered by future microarray trials.^52,71Clearly, large, well-designed, multicenter-driven prospectivevalidation trials assessing microarray-based and current standarddiagnostics in parallel are needed.

   Acknowledgements

We thank our technicians for their excellent assistance.

   Footnotes

Submitted December 30, 2004; accepted April 24, 2005.
Prepublished online as Blood First Edition Paper, May 5, 2005;DOI 10.1182/blood-2004-12-4938.

Supported in part by a grant from the German José CarrerasFoundation (DJCS-R00/13). Gene expression studies in the Laboratoryfor Leukemia Diagnostics are further supported in part by RocheDiagnostics, Integrated Cancer Care Unit (ICCU), Basel, Germany.

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: Torsten Haferlach, Laboratory for Leukemia Diagnostics, Department of Internal Medicine III, Ludwig-Maximilians-University, Marchioninistr 15, 81377 Munich; e-mail: torsten.haferlach{at}med.uni-muenchen.de.

   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