Blood online
Home About Blood Authors Subscriptions Permission Advertising Public Access contact us
 

 
Advanced
Current Issue
First Edition
Future Articles
Archives
Submit to Blood
Search
American Society of Hematology
Meeting Abstracts
Email Alerts
 Blood, 1 July 2005, Vol. 106, No. 1, pp. 274-286.
Prepublished online as a Blood First Edition Paper on March 17, 2005; DOI 10.1182/blood-2004-10-3900.

This Article
Right arrow Abstract Freely available
Right arrow Full Text (PDF)
Right arrow Supplemental Materials/Methods, Tables, and Figures
Right arrow All Versions of this Article:
2004-10-3900v1
106/1/274    most recent
Right arrow Alert me when this article is cited
Right arrow Alert me if a correction is posted
Right arrow Citation Map
Services
Right arrow Email this article to a friend
Right arrow Similar articles in this journal
Right arrow Similar articles in PubMed
Right arrow Alert me to new issues of the journal
Right arrow Download to citation manager
Right arrow reprints & permissions
Right arrow Rights and Permissions
Citing Articles
Right arrow Citing Articles via HighWire
Right arrow Citing Articles via CrossRef
Right arrow Citing Articles via Google Scholar
Google Scholar
Right arrow Articles by Soulier, J.
Right arrow Articles by Sigaux, F.
Right arrow Search for Related Content
PubMed
Right arrow PubMed Citation
Right arrow Articles by Soulier, J.
Right arrow Articles by Sigaux, F.
Related Collections
Right arrow Hematopoiesis and Stem Cells
Right arrow Neoplasia
Right arrow Gene Expression
Social Bookmarking
Add to CiteULike   Add to Connotea   Add to Del.icio.us   Add to Digg   Add to Reddit   Add to Technorati  
What's this?

arrow to previous article Previous Article  |  Table of Contents  |  Next Article next article arrow

NEOPLASIA

HOXA genes are included in genetic and biologic networks defining human acute T-cell leukemia (T-ALL)

Jean Soulier, Emmanuelle Clappier, Jean-Michel Cayuela, Armelle Regnault, Marina García-Peydró, Hervé Dombret, André Baruchel, Maria-Luisa Toribio, and François Sigaux

From Institut National de la Santé et de la Recherche Médicale (INSERM) U462 `Lymphocyte et Cancer,' and Molecular Hematology Laboratory, Institut Universitaire d'Hématologie, Hôpital Saint Louis, Paris, France; Centro de Biología Molecular Severo Ochoa, CSIC, Universidad Autónoma de Madrid, Madrid, Spain; and Adult Hematology Department and Pediatric Hematology Department, Hôpital Saint Louis, Paris, France.


   Abstract
Top
 Abstract
Introduction
 Patients, materials, and methods
 Results
 Discussion
 References
 
Using a combination of molecular cytogenetic and large-scale expression analysis in human T-cell acute lymphoblastic leukemias (T-ALLs), we identified and characterized a new recurrent chromosomal translocation, targeting the major homeobox gene cluster HOXA and the TCRB locus. Real-time quantitative polymerase chain reaction (RQ-PCR) analysis showed that the expression of the whole HOXA gene cluster was dramatically dysregulated in the HOXA-rearranged cases, and also in MLL and CALM-AF10-related T-ALL cases, strongly suggesting that HOXA genes are oncogenic in these leukemias. Inclusion of HOXA-translocated cases in a general molecular portrait of 92 T-ALLs based on large-scale expression analysis shows that this rearrangement defines a new homogeneous subgroup, which shares common biologic networks with the TLX1- and TLX3-related cases. Because T-ALLs derive from T-cell progenitors, expression profiles of the distinct T-ALL subgroups were analyzed with respect to those of normal human thymic subpopulations. Inappropriate use or perturbation of specific molecular networks involved in thymic differentiation was detected. Moreover, we found a significant association between T-ALL oncogenic subgroups and ectopic expression of a limited set of genes, including several developmental genes, namely HOXA, TLX1, TLX3, NKX3-1, SIX6, and TFAP2C. These data strongly support the view that the abnormal expression of developmental genes, including the prototypical homeobox genes HOXA, is critical in T-ALL oncogenesis.


   Introduction
Top
 Abstract
 Introduction
Patients, materials, and methods
 Results
 Discussion
 References
 
T-cell acute lymphoblastic leukemias (T-ALLs) are highly malignant tumors representing 10% to 15% of pediatric and 25% of adult ALLs in humans.1,2 T-ALL cells derive from partially differentiated thymocytes. These cells originate from pluripotent progenitors that are progressively committed to the {alpha}{beta} or {gamma}{delta} T-cell lineages in the thymus.3 Somatic V(D)J recombination rearranges the T-cell-receptor (TCR) gene segments, generating protein products that allow cells to pass through several cellular processes, so-called {beta}-selection and selection.4,5 Hence, V(D)J recombination both directly compromises genome integrity and indirectly controls cellular functions considered to be critical for oncogenesis, such as cell cycle, proliferation, and apoptosis.6 However, T-ALLs remain rare, consistent with efficient control mechanisms that can only be overcome by accumulation of oncogenic events. Several classes of proto-oncogenes can be activated by chromosomal rearrangements or epigenetic mechanisms in T-ALL.7-9 The resulting oncoproteins include basic helix-loop-helix proteins (TAL1/SCL, TAL2, LYL1), homeodomain-containing proteins (TLX1/HOX11, TLX3/HOX11L2), and LIM only proteins (LMO1, LMO2), which are likely to be involved in transcription factor complexes.8,10 In addition, chromosomal alterations or DNA mutations can activate genes involved in signal transduction and thymus differentiation, such as NOTCH1 and LCK,11-13 or can lead to gene fusion (MLL-ENL, CALM-AF10, NUP214-ABL1).14-16 Moreover, the CDKN2A/INK4A/ARF tumor suppressor gene is inactivated by deletion or mutation in most T-ALL cases.17,18 Recently, T-ALL classifications based on selected oncogene expression and corresponding microarray gene expression patterns have been reported.19

In the present study, a combination of molecular cytogenetic and large-scale expression analyses allowed us to identify and characterize a new recurrent chromosomal translocation directly targeting and dysregulating the HOXA locus. This new rearrangement extends the catalog of T-cell oncogenes to these prototypical homeobox genes and strongly suggests that HOX dysregulation can be not only a consequence of cancer in humans but also a cause.20 Moreover, we show that HOXA genes can be included in biologic networks that associate oncogenesis and thymocyte differentiation processes. Our data suggest that inappropriate use or perturbation of specific biologic pathways involved in thymic maturation, and ectopic expression of genes, often developmental genes, are critical for T-ALL oncogenesis.


   Patients, materials, and methods
Top
 Abstract
 Introduction
 Patients, materials, and methods
Results
 Discussion
 References
 
Patients, leukemic cells, and annotations

T-ALL was diagnosed in 92 patients who were treated at Saint Louis Hospital (Paris, France). Seven patients were studied at diagnosis and relapse (total 99 T-ALL samples). There were 56 children (median age, 9 years; range, 1-16 years) and 36 adults (median age, 27 years; range, 17-66 years). Informed consent was obtained from the patients or relatives. The study was approved by the Review Board of the Féderation d'Hématologie, Hôpital Saint-Louis, Paris, France. T-ALL diagnosis was based on morphologic and immunophenotypical criteria using flow cytometry and an extended monoclonal antibody panel. Bone marrow samples from healthy donors (n = 4), unpurified thymus cells, and MOLT4, HSB2, CEM, and Jurkat T-cell lines were also included in the study. DNA and RNA were extracted from the cryopreserved leukemic cells. Expression of the main T-ALL oncogene transcripts, TAL1, TLX1, TLX3, LMO1, LMO2, and LYL1, and the SIL-TAL1, CALM-AF10, and NUP214-ABL1 transcripts were analyzed by real-time quantitative polymerase chain reaction (RQ-PCR; shown in Supplemental Figure S1, available on the Blood website; see the Supplemental Materials link at the top of the online article), as described.21 Because TAL1 is highly expressed in erythroblasts,22 10 cases with high expression of erythroid-associated genes (Table S1) were excluded from the final analysis of TAL1 expression to avoid spurious results. MLL and CDKN2A/INK4A/ARF genomic abnormalities were searched for in the HOXA-expressing cases by fluorescent in situ hybridization (FISH; LSI MLL DualColor, VYSIS/ABOTT, Rungis, France, and RP11-149I2 BAC probe, respectively). MLL partners were identified in the 3 MLL-translocated cases using the MLL fusionChip kit (IPSOGEN, Marseille, France). BMI1, NKX3-1, SIX6, TFAP2C, RAG1, and CD8A gene expression was tested by RQ-PCR (see "PCR systems for gene expression analysis" in the Supplemental Materials and methods).

Isolation of normal human thymocyte subsets

Postnatal thymocytes were obtained from thymus samples removed during corrective cardiac surgery in 3 patients aged 1 month to 3 years old.

Thymocyte subpopulations (for a review, see Carrasco et al4) were isolated and analyzed by fluorescence-activated cell sorting (FACS) for purity as previously described.23-26 Briefly, after rosetting to remove CD2bright thymocytes, CD34+ thymocytes were magnetically sorted and then treated with CD1a microbeads to isolate the CD34+CD1a+ cells (Pre-T1, 96.5% purity). The most immature CD34brightCD33lowCD1a- cells (early thymic progenitors [ETPs]), were sorted from the CD1a-depleted fraction with anti-CD33-phycoerythrin (PE) and anti-PE microbeads (94.6% purity).26 The remaining CD34+ CD33-depleted thymocytes corresponded to CD34+CD1a- Pro-T thymocytes (99.4%). Other thymic subpopulations were purified after centrifugation of total thymus cells on stepwise Percoll density gradients as previously described.4,24 Characteristics of these subsets were: Pre-T2 and Pre-T3(E) (not separated here and further referred as Pre-T2/Pre-T3[E]), 99% CD4+CD8{alpha}{beta}-CD3-TCR{alpha}{beta}-; Pre-T3(L), 98% CD4+CD8{alpha}{beta}+CD3-TCR{alpha}{beta}ic; immature DPs (immature double-positive cells), 98% CD4+CD8{alpha}{beta}+CD3-TCR{alpha}{beta}-; DP-TCR{alpha}{beta}low, 63.2% CD4+CD8{alpha}{beta}+CD3lowTCR{alpha}{beta}low; DP-TCR{alpha}{beta}int, CD8{alpha}{beta}+CD4+ CD3intTCR{alpha}{beta}+, 99% purity with 74% CD3int; DP-TCR{alpha}{beta}br, 99.9% CD8{alpha}{beta}+CD4+CD3brTCR{alpha}{beta}br; CD4-SP (CD4 single-positive cells), 97.2% CD4+CD3brTCR{alpha}{beta}br; and CD8-SP, 99.8% CD8{alpha}{beta}+CD3brTCR{alpha}{beta}br; see "Reagents used for human thymocyte subsets isolation" in the Supplemental Materials and methods.

Genomic analysis of the TCRB and HOXA loci

TCRB-flanking FISH probes were prepared from the CTD-3092H9 P1 artificial chromosome (PAC; 5' probe, centromeric) and RP11-368I15 bacterial artificial chromosome (BAC; 3' probe, telomeric). HOXA-flanking FISH probes were prepared from the RP11-167F23 and RP5-1200I23 BACs (telomeric and centromeric of the HOXA locus, respectively). FISH mapping within the HOXA locus was performed using the RP11-163M21, RP11-1132K14, RP11-1025G19, and RP11-1148E13 BACs. Images were captured and analyzed using a DMRXA epifluorescence microscope (Leica), a Plan Apo 63 x/1.32 oil immersion objective lens (0.132 mm/pixel; Leica), a CCD camera (Cohu), and Q-FISH software (Leica). Southern blot analysis of the HOXA locus was performed using a panel of probes shown in Supplemental Materials and methods. Genome information was collected in the UCSC Genome Bioinformatics site (http://genome.ucsc.edu).

For inverse PCR amplification of the TCRB-HOXA breakpoint regions, leukemic gDNAs were digested by the MaeI and MseI restriction enzymes (cases TL43 and TL46, respectively) and ligated at low concentration. The circularized breakpoint-containing fragments were amplified by nested PCR. Primers were 5'-ATACCCCACCACCAACTTG-3' and 5'-ATGTCTTTGTAAGGCTGTTTG-3' (first round PCR), and 5'-CGCGGATCCATGTCACCCACCCTCCA-3' and 5'-CGCGGATCCCAGTACCCACCCCTCTCC-3' (nested PCR). Reciprocal breakpoint sequences were long-range PCR amplified using the forward HOXA primers 5'-GAGCCTCGTGTCTTTCTCC-3' (case TL43) and 5'-GTTCTAGCTCTATTTACTTCTA-3' (case TL46), and a set of reverse J{beta} primers, including 5'-CTGCTCAGCTCTTTTTGCC-3' (case TL43), and 5'-CCTTCCCACCGCTGAGAG-3' (case TL46). Translocation breakpoints and flanking sequences were sequenced both directly and after cloning in the PCR-Script vector (Stratagene, La Jolla, CA).

RQ-PCR analysis of genes from the HOXA locus

Leukemic and control cDNAs were analyzed for expression of the 11 HOXA and EVX1 genes using SYBRgreen reagents (Applied Biosystems, Courtaboeuf, France). Primers are indicated in Supplemental Materials and methods. Results were expressed in Ct of the amplification curve and normalized on the basis of the expression of 2 housekeeping genes, ABL1 and TBP. Because the HOX paralogs share high sequence similarity, primers were carefully designed to avoid cross-priming. The specificity of the amplified fragments was further checked by analyzing the dissociation curves, migration on polyacrylamide gels, and by direct sequencing of the PCR products for at least one product of each type. In most cases, the primers overlap exon boundaries to prevent contamination by gDNA.

Microarray experiments and data analysis

Large-scale expression and analyses were performed on quality-controlled RNAs using the Affymetrix U133A technology, according to standardized procedures at the Strasbourg Genopole national facility. See "Microarray experiments and data analysis" in the Supplemental Materials and methods for details on RNA control and data normalization.

Microarray analyses were performed on the quantile-normalized data using dChip1.3 (http://biosun1.harvard.edu/complab/dchip/) and BRB (http://linus.nci.nih.gov/BRB-ArrayTools.html) software, as described in the Supplemental Materials and methods. LocusLink symbols and ID (http://www.ncbi.nih.gov/entrez/query.fcgi?db=gene) were used when the information was available to label genes corresponding to the probe sets.


   Results
Top
 Abstract
 Introduction
 Patients, materials, and methods
 Results
Discussion
 References
 
A new recurrent chromosomal translocation in T-ALL targets the HOXA locus

In an attempt to identify new oncogenic abnormalities in T-ALL, we carried out an interphasic FISH screening in 15 T-ALL cases that did not show expression of the 3 oncogenes most commonly involved in this type of leukemia (SIL-TAL1, TLX1, and TLX3). We used FISH probes of the T-cell-receptor {beta} genes locus (TCRB) because this locus is often involved in oncogenic rearrangements of T-ALL and considering that the near-telomeric location of TCRB could lead to cryptic translocations. In this way, we identified 2 T-ALL cases (TL43, TL44) with a TCRB translocation (Figure 1A). Cloning of the TL43 translocation identified the HOXA locus as the TCRB partner sequence (Figure 1B-D). The HOXA locus was also involved in the second case (TL44), as demonstrated by FISH and Southern blot (data not shown).

We addressed the hypothesis that this new recurrent translocation could define a homogeneous T-ALL subgroup by analyzing global gene expression on a series of unselected T-ALL samples.



View larger version (33K):
[in this window]
[in a new window]
  		Figure 1.. A new chromosomal translocation involves the TCRB and HOXA loci. (A) A TCRB chromosomal translocation was identified in leukemic cells of patient TL43 by dissociation of TCRB-flanking FISH probes. The centromeric V{beta}-flanking probe (CTD-3092H9) and the telomeric C{beta}-flanking probe (RP11-168I15) were labeled with Texas red and fluorescein isothiocyanate (FITC), respectively. Original magnification, x 63. (B) A 541-bp fragment containing the D{beta}1 breakpoint was produced by circled nested PCR (left lane, the rearranged band is shown by an arrow; right lane, molecular weight marker). (C) Breakpoint and flanking sequences of both derivative chromosomes of the TCRB-HOXA translocation TL43. Recognition sequence signal (RSS) heptamer and putative heptamer-like sequence are indicated according to consensus.27 Untemplated nucleotides (N-diversity) are typed in lowercase. GL indicates germline; der, derivative chromosomes. (D) Schematic representation of the TCRB-HOXA translocation TL43, drawn to scale according to data from the IMGT Information System (http://imgt.cines.fr) and the UCSC Genome Bioinformatics site (http://genome.ucsc.edu/), and to the DNA sequences of the breakpoint regions of the 2 derivative chromosomes. Chromosomes are depicted according to the direction of the TCRB and HOXA gene transcription (except for the EVX1 gene, which is transcribed in the opposite direction as indicated by arrow). Breakpoints are indicated with arrows.

 
Large-scale expression analysis identifies a HOXA-expressing subgroup within HOX-related T-ALL samples

Leukemic cells from a series of 92 patients, including the 2 patients with the newly identified TCRB-HOXA rearrangement, were studied by transcriptome analysis of tumor cells using Affymetrix U133A microarrays. Sample and gene classifications were performed with unsupervised hierarchical methods using a list of 255 probe sets selected on the basis of expression variability and reliability among samples (the general microarray strategy is shown in Figure 2A; see also "Microarray experiments and data analysis" in the Supplemental Materials and methods for probe-set selection and methods). Major clusters of T-ALL were obtained, and significant correlations with the immunologic and oncogene expression annotations allowed definition of major T-ALL oncogenic groups (Figure 2B).

The first branch of the hierarchy (labeled as TAL1-related, TAL_R) includes all samples with SIL-TAL1 rearrangement (P < .001, 16 cases). Cases of this branch are associated with strong TAL1 expression (P < .001, 33 of 40 T-ALL cases with significant TAL1 expression are found in this branch; see also Figure S1). The cell-surface TCR{alpha}{beta} receptor is frequently expressed (P < .001, 16 of 20 {alpha}{beta} T-ALL cases are included in this branch but no {gamma}{delta} cases), in line with previous work connecting SIL-TAL1 rearrangement with {alpha}{beta} T-cell differentiation.19,28,29 Furthermore, this analysis delineates 2 stable subgroups (TAL_RA and TAL_RB) not identified by previous works.

The second branch of the hierarchy includes all cases with TLX1 and TLX3 expression (P < .001 in both cases). All the {gamma}{delta} T-ALL cases are included in this branch (P < .001, 14 cases). In addition to the TLX1- and TLX3-expressing cases, 2 clusters of samples are found in this branch. A first cluster contains 8 cases, including the 2 HOXA-translocated cases. Stability of this cluster was demonstrated by sampling analysis (Figure S2). The genes that mainly define this cluster are HOXA5, HOXA9, HOXA10, and LRIG1, and accordingly, this subgroup of samples was provisionally named the "HOXA-expressing cluster" (Figure 2B). These cases, and the TLX1- and the TLX3-expressing samples, were collectively named the HOX_R group. Another cluster of samples is characterized by strong expression of genes expressed in immature cells (eg, CD34 or LMO2) and frequent lymphoid and myeloid CD13 or CD33 surface antigen coexpression (P < .001, 9 of 14 cases, excluding the TLX3 samples). Considering that oncogenic events are uncharacterized in these cases but probably occurred at an early stage of differentiation (with lymphoid and myeloid potential), this group was provisionally named "Immature group" and constitutes the third major group of T-ALL. Half the TLX3-expressing samples cocluster with cases of this group, due to expression of immature genes.



View larger version (48K):
[in this window]
[in a new window]
  		Figure 2.. Unsupervised hierarchical classification of samples and genes based on expression microarray data. (A) General flowchart describing the sequence of microarray analysis procedures throughout the study. (B) This bidimensional classification was performed using expression data of probe sets selected on expression variability and reliability through the samples (n = 358 probe sets), and exclusion of probe sets highly expressed in bone marrow cells; the resulting list of 255 probe sets is shown in Table S1. The top panel shows a hierarchical tree of samples (columns), sample subgroups, and sample annotations. Major subgroups corresponding to main hierarchy branches are indicated on the tree. MLL indicates cases with MLL rearrangements; TAL_R, TAL1-related cases, with 2 TAL_R subgroups (TAL_RA and TAL_RB); HOX_R, HOX-related cases; the HOXA-expressing cluster of cases is highlighted in red, and the main TLX1- and TLX3-expressing subgroup is indicated; IMMATURE, subgroup of cases characterized by strong expression of genes expressed in immature cells and frequent coexpression of myeloid genes; BM, normal human bone marrow cells. TL is the unique identification number for samples. Sample group annotations: for genomic annotations, S indicates cases with SIL-TAL1 transcripts; E, TLX1-expressing cases, L, TLX3-expressing cases (both also quoted as genomic annotations for simplicity); t, HOXA-rearranged cases; C, cases with CALM-AF10 transcripts; M, cases with MLL rearrangement as detected in these cases by FISH and Southern blot; and N, cases with NUP214-ABL transcripts. *HOXA_R cases without identified rearrangement. For TAL1, LMO1, and LMO2 gene expression, RQ-PCR evaluations of expression are indicated; - indicates cases not annotated to avoid bias due to erythroid contamination (n = 9 cases, including the HOXA-rearranged cases TL46), or not available (n = 2 cases). TAL1 expression was scored for significant increased levels compared to normal thymus level, evaluated from 1 to 5 (moderate to highest levels), and significant LMO1 and LMO2 expressions compared to normal thymus levels are indicated as P (positive); see Figure S1. Immuno indicates immunologic markers: i, immature; 3, cCD3 expression; g, {gamma}{delta} expression; a, {alpha}{beta} expression; and M, myeloid markers (CD13 or CD33 or both). For oncogenic groups, T indicates TAL_R cases; H, HOX_R cases; I, immature cases without TLX3 expression. For TAL_R subgroup annotations, A indicates TAL_RA; and B, TAL_RB. These labels were assigned based on sample annotations and microarray analyses (Figure S2). Group assignment by prediction models was questionable in 2 TAL_RB cases and 3 immature cases and these cases are indicated by boxes (TL25, TL34, TL76, TL77, and TL82; Figure S2D). The "Immature group" label is provisional because oncogenic events are unidentified in this group. In the middle panel, left, hierarchical tree of genes (rows); center, for all samples (columns), relative expression levels are indicated according to the color scale shown on the bottom of the figure (from deep blue, lower expression, to deep red, higher expression); right, rows corresponding to the HOXA genes are indicated. The bottom panel shows magnification of the cluster of genes defining the HOXA-expressing cluster. These cases, and the 5 additional samples with HOXA expression, are indicated by red boxes (HOXA-expressing samples).

 
Therefore, this analysis identifies a "HOXA-expressing cluster" of T-ALL that includes the 2 HOXA-rearranged samples. These cases cluster in the same branch as TLX1 and half the TLX3-related cases, suggesting a biologic link between these leukemias.

Genomic and expression analysis links HOXA expression to TCRB-HOXA, MLL, and CALM-AF10 chromosomal rearrangements

We investigated the 8 cases of the HOXA-expressing cluster defined by the unsupervised hierarchy, and 5 additional samples with detectable HOXA expression (HOXA-expressing samples, n = 13; Figure 2B). FISH, Southern blot, and reverse transcription-PCR (RT-PCR) were performed. Clinical, immunologic, and genetic features of the corresponding patients are indicated in Table 1.


View this table:
[in this window]
[in a new window]
  		Table 1.. Clinical and biologic features of the HOXA-expressing T-ALL cases

 
In line with previous work,30,31 MLL rearrangements were found in 3 cases, which clustered as an independent homogeneous group (Figure 2B). In addition and unexpectedly, 4 HOXA-expressing cases demonstrated a CALM-AF10 translocation, as detected by RT-PCR.

Considering that the HOXA-expressing cases included 2 cases (TL43 and TL44) with a TCRB-HOXA translocation, we searched for additional HOXA rearrangements in this subgroup (Table 1). Two more TCRB-HOXA translocations were identified using FISH (cases TL45 and TL46). The HOXA breakpoint location was mapped by Southern blot analysis in the 4 cases, and the TL46 translocation was fully characterized by sequencing of the 2 derivative breakpoint regions, in addition to case TL43 (Figure S3). Strikingly, the 4 breakpoints clustered in a genomic region of 2.6-kb length located between the HOXA10 and HOXA9 genes (BCRHOXA; Figure 3A). In the final 2 HOXA-expressing cases (TL47 and TL48), no HOXA rearrangement was detected, suggesting additional mechanisms of HOXA activation, as has also been reported for TAL1 and TLX1 activation.35-37 The 4 TCRB-HOXA cases were collectively named the HOXA-related (HOXA_R) subgroup, along with cases TL47 and TL48, because these 2 cases most frequently clustered with HOXA-rearranged cases in clustering experiments (Figure S2).

To analyze the consequence of the translocations on the expression of the HOXA locus, all 11 HOXA genes, as well as the non-HOX homeobox gene EVX1 located in the vicinity of the HOXA locus, were analyzed for expression using specific RQ-PCR. All cases with TCRB-HOXA, CALM-AF10, and MLL rearrangements consistently demonstrated global overexpression of most HOXA genes (but no EVX1 deregulation), compared to levels in normal thymus and control T-ALLs (Figure 3B). Strikingly, HOXA genes located on both sides of the TCRB-HOXA breakpoints were overexpressed. In addition, whereas we failed to amplify any potential TCRB-HOXA fusion transcript (data not shown), we found that a HOXA10 gene transcript, referred to as HOXA10B, was present at high levels in all the 4 HOXA-rearranged cases and in the 2 additional HOXA_R cases (Figure 3B). By contrast, no consistent expression of this HOXA10B transcript was detected in the thymus and other samples.

Therefore, the combination of large-scale expression, molecular cytogenetic, and gene-specific expression analyses allowed detailed description of the new recurrent HOXA chromosomal rearrangement. This rearrangement strongly deregulates the HOXA multigene cluster. In addition, a new association was detected between the CALM-AF10 rearrangement and expression of HOXA genes.

Inclusion of HOXA-expressing cases in a general molecular portrait of T-ALL

To analyze gene pathways differentially involved in T-ALL (including those of the HOXA_R subgroup), we studied expression profiles of the oncogenic T-ALL groups. First, a compendium of 469 probe sets differentially expressed between the previously defined T-ALL groups was obtained (see "Microarray experiments and data analysis" in the Supplemental Materials and methods). Then, a supervised hierarchical classification of the genes was performed, allowing definition of 13 gene clusters based on correlated expression in the T-ALL groups (Figure 4; Table S2 provides a list of genes and clusters). Tentative examination of the known biologic function of the genes shows that a high number of them are linked to thymocyte differentiation or general cellular functions like signaling, cell cycle, DNA repair, and antiapoptotic pathways.

As expected, the HOXA_R, CALM-AF10, and MLL cases express a cluster of genes containing HOXA5, HOXA9, HOXA10, and HOXA11 (cluster C9; Figure 4B). HOXA_R cases are also characterized by high average expression of genes, which have been involved in T-cell differentiation or oncogenesis (or both), including NOTCH2, NOTCH3, PTCRA (Pre-T{alpha} gene), TCRG, TCRD, and PIM1 (clusters C7, C8, and C11), also shared with the TLX1 and TLX3 subgroups. Together with the fact that HOXA-rearranged, TLX1-, and most of the TLX3-expressing cases cluster in the unsupervised hierarchy (Figure 2B), these data reinforce the view that these subgroups share biologic similarities by using common pathways involved in thymocyte differentiation and, most likely, in T-cell oncogenesis.



View larger version (42K):
[in this window]
[in a new window]
  		Figure 3.. Clustering of the breakpoints and dysregulated expression of the HOXA genes in leukemias with TCRB-HOXA rearrangement. (A) The 4 breakpoints cluster in a 2.6-kb breakpoint cluster region (BCRHOXA) as indicated. The direction of transcription is shown by arrows (centromere to telomere for the HOXA genes, and opposite direction for EVX1). Transcription products of the HOXA genes are drawn according to the data of the UCSC site. The HOXA10B exons are shown as red boxes. The rearrangements disrupt the HOXA locus at the 3' end of HOXA10 gene (cases TL44, TL45, and TL46), and within the intron Ib region of HOXA9 (TL43), as indicated. Open reading frames are shown as black boxes. The 2 isoforms of the HOXA10 protein (HOXA10A, quoted HOXA10, and HOXA10B) are drawn according to previous reports, and the homeobox DNA-binding domain is indicated.32-34 (B) Analysis of expression of the HOXA genes by specific real-time RT-PCR in T-ALL samples. The HOXA and EVX1 expression values are shown in the 4 HOXA-rearranged cases (marked t), and the 2 HOXA-related cases without detected chromosomal rearrangement (TL47 and TL48, marked *), which constitute the HOXA_R group. Values in the 3 MLL-rearranged cases, the 4 CALM-AF10 cases, a panel of TAL_R and TLX1/TLX3 samples, T-cell lines, normal human thymus, and normal bone marrow samples are shown. HOXA9B and HOXA10B transcripts were also analyzed (bottom rows). Median normalized Ct values are indicated and a color scale was used as shown.

 
In addition to the expression of HOXA genes, the CALM-AF10- and MLL-related cases are characterized by a high expression of the BMI1 gene (Figure 4B; BMI1 expression was confirmed by specific RQ-PCR, not shown). Bmi1 has been implicated in experimental murine B-cell leukemias38 and in self-renewal of normal and leukemic stem cells.39 This gene is considered a repressor of the HOX genes,40 which contrasts intriguingly with the high expression of HOXA genes in the MLL- and CALM-AF10-related cases (Figure 4B).

By comparison with the HOXA_R samples, and more generally with the HOX_R group, samples from the immature group strongly express the LMO2, LYL1, CD34, BCL2, FLT3, and TGFB1 genes (cluster C10, "hematopoiesis") but have low expression of genes from other clusters, particularly from cluster C6, which appears linked to "proliferation and mitosis," whereas there is a variable expression of this cluster throughout samples in the other groups (Figure 4A). Half the TLX3-expressing cases coexpress genes characteristic of both the immature and HOX_R groups, and accordingly these cases cluster with immature cases. Samples from the TAL_R group express genes involved in TCRB signaling (cluster C3), particularly in the TAL_RB samples. In addition, the TAL_RB samples share with HOX_R cases (particularly TLX1 cases) a high expression of T-cell differentiation genes (cluster C4 and C7), including NOTCH3 and PTCRA. Samples from the TAL_RA subgroup specifically express the signaling genes STAT5A and STAM1 (cluster C2). Interestingly, numerous genes not normally expressed in thymus have ectopic expression in TAL_R samples, including 2 homeobox genes, NKX3-1 and SIX6.

Analysis of oncogenic T-ALL subgroups with respect to normal T-cell differentiation

At this point, we analyzed gene expression in T-ALL samples with respect to normal thymic differentiation. For this purpose, 11 distinct thymic subpopulations were purified from normal human thymus, and global gene expression analysis using U133A microarrays was performed. The 469 probe sets differentially expressed between oncogenic groups (Figure 4A) were filtered for thymic expression and proliferation genes were excluded, resulting in 168 genes (see "Microarray experiments and data analysis" in the Supplemental Materials and methods).

First, an unsupervised hierarchy of the thymic subpopulations and the 168 genes was performed. Importantly, the sample classification recapitulates the sequential steps of thymocyte differentiation (Figure 5A). Moreover, examination of the gene clusters of normal thymic subpopulations frequently shows similar patterns compared to gene clusters of T-ALL (compare Figures 4A and 5A), pinpointing networks whose coordinated expression is conserved in leukemic cells (ie, FLT3-LMO2-CD34-LYL1 and CD1A-CD8A-RAG1). In rarer cases, different gene clustering suggests that abnormal coexpression in T-ALL samples could be important in the oncogenic process. For instance, PTCRA and NOTCH3 are coexpressed in subgroups of T-ALL samples, including HOX_R samples (Figure 4A), whereas in normal thymic subpopulations PTCRA is expressed at the highest level before the {beta}-selection process and NOTCH3 afterward (Figure 5A).



View larger version (73K):
[in this window]
[in a new window]
  		Figure 4.. Supervised clustering of genes differentially expressed among major sample groups. (A) This hierarchical classification was performed using 469 probe sets detecting differential expression among sample groups (Figure 2A). Samples were preclassified according to oncogenic group assignment as defined in Figure 2B. The same conventions for sample annotations are used. The HOXA_R subgroup is indicated (HOXA-rearranged, n = 4, and HOXA-related, n = 2). Clusters of genes defined by this supervised clustering are indicated (clusters 0-12). Genes of particular interest are labeled using Locuslink symbol, and genes without significant thymic expression are highlighted in yellow (ectopic thymic expression). The cluster C9, which is defined by HOXA-expressing samples and contains HOXA genes, is highlighted in red. (B) List of genes from clusters C8 and C9 and relative expression in oncogenic subgroups. Genes from cluster C8 are frequently highly expressed in subsets from the HOX_R group; cluster C9 is defined mainly by the HOXA-expressing samples (HOXA_R, CALM-AF10, and MLL) and includes HOXA genes (in red); "ectopic" genes with respect to thymus expression are highlighted in yellow. NA indicates Locuslink symbol not available. Relative expression in each T-ALL group is shown by color scale.

 
Then, by analyzing leukemic samples using the 168 "thymic genes," we found that a consistent hierarchy of T-ALL could be obtained (Figure 5B; compare with Figure 2B). Therefore, to define the differentiation stages of leukemic cells according to biologic pathways, T-ALL and thymic subpopulations data were combined. Hierarchical analysis and multidimensional scaling visualization were performed and informative coclustering of T-ALL subgroups and thymic subsets was observed (Figure 5C-D). The HOXA_R samples cluster with the Pre-T1 and Pre-T2/Pre-T3(E) subpopulations, together with the TLX1- and half the TLX3-expressing samples. Therefore, these samples appear arrested at a stage corresponding to T-lineage engagement preceding the {beta}-selection process. By contrast, the TAL_R samples cluster with subpopulations corresponding to steps following {beta}-selection. Samples from the immature group, as well as the CALM-AF10, MLL, and half the TLX3-expressing leukemic samples, cluster with the most immature ETP and Pro-T subpopulations, which correspond to the lineage choice process. Notably, further examination of gene expression in leukemic samples with respect to normal subpopulations reveals numerous abnormalities in the differentiation process (in addition to the differentiation arrest itself). For instance, a few HOX_R samples, including 2 TCRB-HOXA cases, unexpectedly coexpress CD10/MME and TCR{alpha}{beta} heterodimer (Figure 4B). Strikingly, numerous T-cell differentiation-associated genes are expressed at dramatically lower levels in T-ALL samples compared with the relevant normal thymic subpopulations, such as CD8A, RAG1, CD1s, PTCRA, and TCRA in the TAL-R cases (Figure 5C; CD8A and RAG1 expression was confirmed in thymic subsets and T-ALL samples using RQ-PCR, not shown). Conversely, several genes are expressed at higher levels in T-ALL than in normal thymic subsets, such as STAT5A in TAL_RA cases.

Oncogenic groups of T-ALL can be classified using "ectopic" gene expression

Because subgroups of T-ALL can be easily classified by genes normally expressed during thymic differentiation, we wondered whether the unsupervised clustering of T-ALL samples defined in this work merely reflects the differentiation status of the cells, or whether it may also specifically highlight oncogenic events. The 469 probe sets differentially expressed between oncogenic groups (Figure 4A) were filtered for ectopic expression with reference to expression in normal thymic subpopulations and bone marrow (considering that a fraction of T-ALL cells coexpress immature and myeloid-associated genes), resulting in a working list of 23 "ectopic" genes (see "Microarray experiments and data analysis" in the Supplemental Materials and methods). An unsupervised classification of the leukemic samples was performed using these genes. Strikingly, the resulting hierarchy properly classifies the major T-ALL oncogenic subgroups (Figure 6).

Importantly, this gene-filtering strategy was able to select the TLX1 and TLX3 genes and a HOXA gene (HOXA11), all genes that can be targeted by chromosomal translocations as demonstrated here for the HOXA locus. Note, however, that some genes linked to oncogenesis were excluded due to their expression in certain thymic subpopulations or in bone marrow, such as TAL1, LMO2, and the HOXA genes except HOXA11. Interestingly, 2 homeobox genes, NKX3-1 and SIX6, are included in the list of ectopic genes, and they are expressed in TAL_R cases. Notably, a gene related to NKX3-1, namely NKX2-5, has been involved in chromosomal translocations in T-cell lines.41 Additional genes involved in development or morphogenesis were also selected, including TFAP2C and GDF10 (BMP family). Expression level of NKX3-1, SIX6, and TFAP2C was confirmed by specific RQ-PCR in representative T-ALL samples. It therefore appears that ectopic expression of at least one developmental gene is found in most leukemic cases from the major HOX_R and TAL_R groups.

These results demonstrate that the subgroups of T-ALL are not only defined by their differentiation status but also by ectopic expression of genes, including developmental genes.


   Discussion
Top
 Abstract
 Introduction
 Patients, materials, and methods
 Results
 Discussion
References
 
The HOXA gene cluster is an oncogenic target in T-ALL

By combining molecular cytogenetic and expression analysis approaches, we have identified and characterized a new recurrent molecular rearrangement involving the HOXA and TCRB loci in T-ALL. Interphasic FISH patterns and breakpoint sequencing were consistent with chromosomal inversion inv(7)(p15q34) in cases TL44, TL45 and TL46, and translocation t(7;7)(p15;q34) in case TL43 (no karyotypic data were available). Notably, such chromosomal rearrangements have been recurrently reported in T-ALL,42 (see also http://cgap.nci.nih.gov/Chromosomes/Mitelman), but it was probably assumed that they would always reproduce in T-ALL the TCRG-TCRB rearrangements frequently found in T cells in patients with ataxia-telangiectasia.43,44



View larger version (61K):
[in this window]
[in a new window]
  		Figure 5.. Unsupervised clustering of human thymocyte subpopulations and leukemic cells. (A) Unsupervised classification of 11 subpopulations purified from normal human thymus and subsequently analyzed by global gene expression on the U133A array. For human thymic subsets, ETP indicates early thymocyte precursor with lymphomyeloid potential25,26; the Pro-T, Pre-T1, Pre-T2/Pre-T3(E) (ie, Pre-T2 and Pre-T3(E), not distinguished here), Pre-T3(L), immature DP (immature double-positive cells), DP-TCR{alpha}{beta}lo, DP-TCR{alpha}{beta}int and DP-TCR{alpha}{beta}br, CD4-SP (CD4 single-positive cells), and CD8-SP, have been described previously (for a review, see Carrasco et al4). The lineage choice, {beta}-selection, and selection processes as reported in normal thymus differentiation are indicated. The 469 probe sets differentially expressed between oncogenic groups (Figure 4A) were filtered for variable and reliable thymic expression. In addition, "proliferation genes" defined by the "proliferation-mitosis" cluster (cluster C6 in Figure 4A) were discarded from this analysis to avoid spurious sample clustering due to proliferation rate. The resulting final list of 168 "thymic" genes is shown in Table S3. Genes of particular interest are shown, and HOXA genes are indicated in red. (B) Unsupervised classification of T-ALL samples using the same 168 "thymic" gene list. The same conventions are used as in Figure 2. The main oncogenic subgroups are indicated. The same genes of interest as in Figure 5A are shown. (C) Unsupervised analysis of combined T-ALL samples, normal human thymic subpopulations, and bone marrow (BM) cells. A selection of genes with a strongly altered expression level compared with the corresponding normal thymic subsets is indicated (RAG1 and CD8A gene expression was also directly analyzed by RQ-PCR in normal thymic samples and T-ALL, giving consistent data; not shown). (D) Three-dimensional representation of a multidimensional scaling analysis performed using normal thymic subsets, normal bone marrow, and T-ALL samples of the main oncogenic subgroups (TAL_RA, TAL_RB, HOXA, TLX1, TLX3, immature). The lineage choice, {beta}-selection, and selection processes are indicated.

 



View larger version (70K):
[in this window]
[in a new window]
  		Figure 6.. Unsupervised clustering of T-ALL samples based on `ectopic' genes. The 469 probe sets differentially expressed between oncogenic groups (Figure 4A) were filtered for ectopic expression with reference to expression in normal thymic subpopulations and bone marrow, resulting in a working list of 23 ectopically expressed genes. Genes known to be involved in development are boxed. The main T-ALL oncogenic subgroups and annotations are indicated as in other figures.

 
The HOXA gene cluster is one of the 4 major homeobox gene clusters. Each cluster displays 9 to 11 paralogous HOX genes, with a conserved structural organization and a tightly regulated expression.45-48 We found that the disruption of the HOXA locus by TCRB chromosomal rearrangements was associated with a global overexpression of the HOXA genes (Figure 3B). This may be due to the juxtaposition of TCRB regulatory elements in the vicinity of the HOXA genes7,49 and also to the separation of the locus into 2 parts, which may disrupt the normal regulatory elements of the cluster. Alternatively, nonconventional deregulation mechanisms involving miRNA might also be involved50 or, at a higher level, the new chromosome structure resulting from the rearrangement might induce global changes in the nucleus and chromatin organization.51 Interestingly, the 4 HOXA breakpoints cluster tightly at the vicinity of the HOXA10 and HOXA9 genes (Figure 3A). Whereas we could not detect a TCRB-HOXA fusion transcript, strong expression of an alternative transcript known as the HOXA10B transcript was detected in addition to the global HOXA gene overexpression (Figure 3A-B). This transcript, also called the HOXA10 short transcript, has been found in embryonic cells and myeloid cell lines but not in normal hematopoiesis.32,33,52 It encodes a short protein that contains the HOXA10 homeobox DNA-binding domain but lacks the N-terminal regulatory region and that may have distinct functional properties.33,34 The TCRB-HOXA translocation is, to our knowledge, the first example of a recurrent chromosomal rearrangement associated with such a direct and major dysregulation of a multigenic locus.

MLL-translocated cases of the present series demonstrate a strong expression of the HOXA genes, consistent with previous reports.30,31 The direct targeting of the HOXA locus by chromosomal rearrangement strongly supports the hypothesis that dysregulation of HOXA gene expression, triggered by MLL fusion proteins, is causal in MLL-related oncogenesis, consistent with in vitro properties of MLL proteins.53-56 The fact that MLL and HOX_R groups do not cluster in unsupervised hierarchy may suggest that additional genes targeted by the MLL fusions could play an important role in oncogenesis. A major oncogenic role of HOXA genes in T-ALL with CALM-AF10 translocation is also suggested by our results.

The HOX gene network is involved in embryogenesis, stem cell renewal, cell fate, and control of cell differentiation in many tissue types including hematopoietic system and thymus.45,57-60 The evidence increasingly suggests that HOX genes might play a central role in oncogenesis, including in leukemia.2,20,58,61-65 In myeloid leukemias, several HOX genes including HOXA9 can be involved in gene fusion with NUP98, leading to chimeric proteins.66-68 The present identification of the TCRB-HOXA rearrangement in human leukemia, involving the prototypical homeobox genes HOXA, strongly reinforces the view that abnormal expression of developmental genes can be causal in human cancer.

Large-scale expression analysis defines complete typology of T-ALL

Unsupervised classifications allow definition of the overall typology of samples, without a priori knowledge of the sample annotations.69 New homogeneous subgroups can be identified using these methods, as shown here in the HOXA-rearranged cases. Importantly, comparison of the sample annotations with the distinct oncogenic groups in our series of 92 cases suggests that a complete model of T-ALL has been here delineated. Major stable groups have been defined by unsupervised analysis on a large number of samples and genes, and this classification makes sense because it pinpoints links between these groups and genetic rearrangements, ectopic expression of genes including known oncogenes, and critical stages of thymus differentiation. It is therefore likely that potential new subgroups in T-ALL would represent discreet variations within these major groups or rare distinct subgroups.

Using a supervised approach based on oncogene expression, Ferrando et al identified a set of genes differentially expressed in T-ALL samples.19 An unsupervised classification of our samples using a list of genes based on this set properly classifies the major oncogenic groups (Figure S4). It is likely that the LYL1 group defined in this previous work partially overlaps with our provisionally named immature group (note, however, that LYL1 is expressed in the corresponding normal thymic immature subpopulation). Importantly, 3 cases here identified as HOXA-translocated cocluster using this former set of genes, within a branch containing the vast majority of TLX1 and TLX3 cases (Figure S4). Comparison of these 2 studies demonstrates the reliability of the gene expression approach and emphasizes the view that TCRB-HOXA-rearranged cases represent a homogeneous T-ALL subgroup.

HOXA genes are included in biologic networks that connect oncogenesis, thymic differentiation pathways, and ectopic gene expression

Important data were obtained by analyzing expression profiles of leukemic samples with respect to those of normal human thymocyte subpopulations. Although oncogenic processes dramatically alter levels of gene expression, we found that conserved gene expression networks allow pertinent coclustering of leukemic and thymic samples (Figure 5C). T-ALL cells of the major groups (TAL_R, HOX_R, and immature) appear arrested at distinct stages of differentiation, as previously suggested,19,28,29,70 corresponding to critical events in thymic maturation. Specifically, the HOXA-rearranged and TLX1-expressing cases closely match differentiation stages of Pre-T1 to Pre-T2/Pre-T3(E) subsets, whereas TLX3-expressing cases extend from ETP to Pre-T2/Pre-T3(E), all stages preceding the {beta}-selection process. This correlation between oncogene expression and arrest at precise stages of differentiation may suggest that expression of distinct oncogenes is associated with the inhibition of distinct differentiation pathways. For instance, it has been reported that ectopic expression of TAL1 oncoprotein may perturb T-cell differentiation by disturbing the expression of E2A target genes.71-73 Consistently, we found in TAL_R samples that many genes characteristic of steps later than {beta}-selection have dramatic underexpression, although these samples cocluster with thymic subpopulations corresponding to these late stages (Figure 5C). It therefore appears that these samples do not display a complete {beta}-selection pattern. One can hypothesize that protection mechanisms have been selected in evolution to avoid the generation of tumors at this stage normally associated with pre-TCR signaling and a resulting high proliferation rate. For instance, RAG2 phosphorylation inhibits V(D)J recombination in cycling thymocytes,74 and this may protect highly proliferative cells in {beta}-selection from a major mechanism of oncogenic chromosomal rearrangement.

Once arrested, leukemic cells might continuously activate certain biologic pathways normally transiently used at these stages, like antiapoptotic pathways. In addition, we found a distortion in expression of certain genes critical for thymic differentiation. For instance, NOTCH2, NOTCH3, and PTCRA genes are coexpressed in most human T-ALL cases (Figure 4A), as reported.75 Interestingly, these genes cocluster in T-ALL samples but not in normal thymic subpopulations, suggesting that an abnormal coexpression of these genes could be specifically associated with oncogenesis. Consistent with a major oncogenic role of the activated NOTCH genes, NOTCH1 is frequently targeted by activating mutations (or rare chromosomal translocation) in human T-ALL,11,13 and expression of a constitutively active intracellular domain of Notch3 favors murine T-cell leukemia in a Ptcra-dependent manner.75 Interestingly, 2 of the 4 HOXA-rearranged cases here identified also have prototypical NOTCH1 DNA mutation (leading to L1601P and H1602L+1603insP mutated proteins in cases TL43 and TL45, respectively, data not shown), demonstrating that HOXA and NOTCH1 genomic abnormalities can be associated and probably cooperate in these cases.

Finally, it appears from our data that a number of genes, including developmental genes, have abnormal, frequently ectopic, expression in certain T-ALL samples compared with normal thymic subpopulations. These include HOXA, TLX1, and TLX3 genes, which can be targeted by recurrent chromosomal translocation as demonstrated here for the HOXA genes, and CDKN2A/INK4A/ARF, frequently inactivated by DNA mutation or deletion as a tumor suppressor gene.17,18 Ectopic expression in T-ALL samples of other developmental genes, such as NKX3-1, SIX6, and TFAP2C suggests that these genes might also be involved in T-ALL oncogenesis (Figure 6). Interestingly, expression of some of these genes has been previously linked to cancer.76,77 Notably, both the NKX2-5 gene (homeobox gene paralogous to NKX3-1) and the TAL1 gene are targeted by chromosomal rearrangements in the T-ALL cell line CEM-CCRF, suggesting potential oncogenic cooperation.41 Altogether, our results are consistent with a model in which developmental genes, including the prototypical HOXA genes in some leukemia subgroups, play a central role in T-ALL oncogenesis.63


   Acknowledgements
 
This paper reports data of the pilot project of the Carte d'Identité des Tumeurs program from the Ligue National Contre le Cancer.

We thank all physicians who sent leukemic samples to the Hematology Laboratory, and especially Thierry Leblanc and Emmanuel Raffoux. We gratefully thank F.A.B. members Georges Flandrin and Marie-Thérèse Daniel for expert morphologic evaluation of leukemic samples. We thank the Xavier Fund for RNA extraction and contribution to oncogene expression analysis, Marie Romeo for CALM-AF10 and BMI1 transcript evaluation, Claire Pichereau for contribution to FISH analysis, and Antoine Crinquette for contribution to Southern blot experiments. We thank Philippe Dessen (Institut Gustave Roussy, Villejuif, France) for updates of gene annotations. We also thank Christelle Thibault, Philippe Kastner, and Doulaye Dembelé (Strasbourg Genopole National Facility, Illkirch, France), Fabien Patel (CIT program, Ligue Nationale contre le Cancer), and Elisabeth Savariau and Robin Nancel (Service d'Infographie, Institut Universitaire d'Hématologie, Paris). We thank Catharine M. Green, Jacques Haiech, Alain Aurias, and Didier Auboeuf for critical comments on the manuscript.


   Footnotes
 
Submitted October 7, 2004; accepted February 27, 2005.

Prepublished online as Blood First Edition Paper, March 17, 2005; DOI 10.1182/blood-2004-10-3900.

Supported by grants from the Ligue Nationale contre le Cancer (`Programme Cartes d'Identité des Tumeurs'), the Ministère de la Recherche (`Programme Génomique'), the Ministère de la Santé (`Programme Tumorothèques'), and INSERM.

The online version of the article contains a data supplement.

The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.

Reprints: François Sigaux, INSERM U462, Institut Universitaire d'Hématologie, Centre Hayem, Hôpital Saint Louis, 1 Ave Claude Vellefaux, 75010 Paris, France; e-mail: fs{at}chu-stlouis.fr.


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

  1. Boucheix C, David B, Sebban C, et al. Immunophenotype of adult acute lymphoblastic leukemia, clinical parameters, and outcome: an analysis of a prospective trial including 562 tested patients (LALA87). French Group on Therapy for Adult Acute Lymphoblastic Leukemia. Blood. 1994;84: 1603-1612.[Abstract/Free Full Text]

  2. Pui CH, Relling MV, Downing JR. Acute lymphoblastic leukemia. N Engl J Med. 2004;350: 1535-1548.[Free Full Text]

  3. Spits H, Blom B, Jaleco AC, et al. Early stages in the development of human T, natural killer and thymic dendritic cells. Immunol Rev. 1998;165: 75-86.[CrossRef][Medline] [Order article via Infotrieve]

  4. Carrasco YR, Navarro MN, de Yebenes VG, Ramiro AR, Toribio ML. Regulation of surface expression of the human pre-T cell receptor complex. Semin Immunol. 2002;14: 325-334.[CrossRef][Medline] [Order article via Infotrieve]

  5. Spits H. Development of alphabeta T cells in the human thymus. Nat Rev Immunol. 2002;2: 760-772.[CrossRef][Medline] [Order article via Infotrieve]

  6. Hanahan D, Weinberg RA. The hallmarks of cancer. Cell. 2000;100: 57-70.[CrossRef][Medline] [Order article via Infotrieve]

  7. Rabbitts TH. Chromosomal translocations in human cancer. Nature. 1994;372: 143-149.[CrossRef][Medline] [Order article via Infotrieve]

  8. Ferrando AA, Look AT. Clinical implications of recurring chromosomal and associated molecular abnormalities in acute lymphoblastic leukemia. Semin Hematol. 2000;37: 381-395.[CrossRef][Medline] [Order article via Infotrieve]

  9. Bernard OA, Busson-LeConiat M, Ballerini P, et al. A new recurrent and specific cryptic translocation, t(5;14)(q35;q32), is associated with expression of the Hox11L2 gene in T acute lymphoblastic leukemia. Leukemia. 2001;15: 1495-1504.[CrossRef][Medline] [Order article via Infotrieve]

  10. Rabbitts TH. LMO T-cell translocation oncogenes typify genes activated by chromosomal translocations that alter transcription and developmental processes. Genes Dev. 1998;12: 2651-2657.[Free Full Text]

  11. Ellisen LW, Bird J, West DC, et al. TAN-1, the human homolog of the Drosophila notch gene, is broken by chromosomal translocations in T lymphoblastic neoplasms. Cell. 1991;66: 649-661.[CrossRef][Medline] [Order article via Infotrieve]

  12. Tycko B, Smith SD, Sklar J. Chromosomal translocations joining LCK and TCRB loci in human T cell leukemia. J Exp Med. 1991;174: 867-873.[Abstract/Free Full Text]

  13. Weng AP, Ferrando AA, Lee W, et al. Activating mutations of NOTCH1 in human T cell acute lymphoblastic leukemia. Science. 2004;306: 269-271.[Abstract/Free Full Text]

  14. Rubnitz JE, Camitta BM, Mahmoud H, et al. Childhood acute lymphoblastic leukemia with the MLL-ENL fusion and t(11;19)(q23;p13.3) translocation. J Clin Oncol. 1999;17: 191-196.[Abstract/Free Full Text]

  15. Asnafi V, Radford-Weiss I, Dastugue N, et al. CALM-AF10 is a common fusion transcript in T-ALL and is specific to the TCRgammadelta lineage. Blood. 2003;102: 1000-1006.[Abstract/Free Full Text]

  16. Graux C, Cools J, Melotte C, et al. Fusion of NUP214 to ABL1 on amplified episomes in T-cell acute lymphoblastic leukemia. Nat Genet. 2004;36: 1084-1089.[CrossRef][Medline] [Order article via Infotrieve]

  17. Cayuela JM, Madani A, Sanhes L, Stern MH, Sigaux F. Multiple tumor-suppressor gene 1 inactivation is the most frequent genetic alteration in T-cell acute lymphoblastic leukemia. Blood. 1996;87: 2180-2186.[Abstract/Free Full Text]

  18. Gardie B, Cayuela JM, Martini S, Sigaux F. Genomic alterations of the p19ARF encoding exons in T-cell acute lymphoblastic leukemia. Blood. 1998;91: 1016-1020.[Abstract/Free Full Text]

  19. Ferrando AA, Neuberg DS, Staunton J, et al. Gene expression signatures define novel oncogenic pathways in T cell acute lymphoblastic leukemia. Cancer Cell. 2002;1: 75-87.[CrossRef][Medline] [Order article via Infotrieve]

  20. Abate-Shen C. Deregulated homeobox gene expression in cancer: cause or consequence? Nat Rev Cancer. 2002;2: 777-785.[CrossRef][Medline] [Order article via Infotrieve]

  21. Gabert J, Beillard E, van der Velden VH, et al. Standardization and quality control studies of `real-time' quantitative reverse transcriptase polymerase chain reaction of fusion gene transcripts for residual disease detection in leukemia—a Europe Against Cancer program. Leukemia. 2003;17: 2318-2357.[CrossRef][Medline] [Order article via Infotrieve]

  22. Delabesse E, Bernard M, Meyer V, et al. TAL1 expression does not occur in the majority of T-ALL blasts. Br J Haematol. 1998;102: 449-457.[CrossRef][Medline] [Order article via Infotrieve]

  23. Ramiro AR, Trigueros C, Marquez C, San Millan JL, Toribio ML. Regulation of pre-T cell receptor (pT alpha-TCR beta) gene expression during human thymic development. J Exp Med. 1996;184: 519-530.[Abstract/Free Full Text]

  24. Carrasco YR, Trigueros C, Ramiro AR, de Yebenes VG, Toribio ML. Beta-selection is associated with the onset of CD8beta chain expression on CD4(+)CD8alphaalpha(+) pre-T cells during human intrathymic development. Blood. 1999;94: 3491-3498.[Abstract/Free Full Text]

  25. de Yebenes VG, Carrasco YR, Ramiro AR, Toribio ML. Identification of a myeloid intrathymic pathway of dendritic cell development marked by expression of the granulocyte macrophage-colony-stimulating factor receptor. Blood. 2002;99: 2948-2956.[Abstract/Free Full Text]

  26. Garcia-Peydro M, de Yebenes VG, Toribio ML. Sustained Notch1 signaling instructs the earliest human intrathymic precursors to adopt a gammadelta T-cell fate in fetal thymus organ culture. Blood. 2003;102: 2444-2451.[Abstract/Free Full Text]

  27. Marculescu R, Le T, Simon P, Jaeger U, Nadel B. V(D)J-mediated translocations in lymphoid neoplasms: a functional assessment of genomic instability by cryptic sites. J Exp Med. 2002;195: 85-98.[Abstract/Free Full Text]

  28. Macintyre EA, Smit L, Ritz J, Kirsch IR, Strominger JL. Disruption of the SCL locus in T-lymphoid malignancies correlates with commitment to the T-cell receptor alpha beta lineage. Blood. 1992;80: 1511-1520.[Abstract/Free Full Text]

  29. Asnafi V, Beldjord K, Libura M, et al. Age-related phenotypic and oncogenic differences in T-acute lymphoblastic leukemias may reflect thymic atrophy. Blood. 2004;104: 4173-4180.[Abstract/Free Full Text]

  30. Armstrong SA, Staunton JE, Silverman LB, et al. MLL translocations specify a distinct gene expression profile that distinguishes a unique leukemia. Nat Genet. 2002;30: 41-47.[CrossRef][Medline] [Order article via Infotrieve]

  31. Ferrando AA, Armstrong SA, Neuberg DS, et al. Gene expression signatures in MLL-rearranged T-lineage and B-precursor acute leukemias: dominance of HOX dysregulation. Blood. 2003;102: 262-268.[Abstract/Free Full Text]

  32. Lawrence HJ, Sauvageau G, Ahmadi N, et al. Stage- and lineage-specific expression of the HOXA10 homeobox gene in normal and leukemic hematopoietic cells. Exp Hematol. 1995;23: 1160-1166.[Medline] [Order article via Infotrieve]

  33. Benson GV, Nguyen TH, Maas RL. The expression pattern of the murine Hoxa-10 gene and the sequence recognition of its homeodomain reveal specific properties of abdominal B-like genes. Mol Cell Biol. 1995;15: 1591-1601.[Abstract]

  34. Eklund EA, Jalava A, Kakar R. Tyrosine phosphorylation of HoxA10 decreases DNA binding and transcriptional repression during interferon gamma-induced differentiation of myeloid leukemia cell lines. J Biol Chem. 2000;275: 20117-20126.[Abstract/Free Full Text]

  35. Bash RO, Hall S, Timmons CF, et al. Does activation of the TAL1 gene occur in a majority of patients with T-cell acute lymphoblastic leukemia? A Pediatric Oncology Group study. Blood. 1995;86: 666-676.[Abstract/Free Full Text]

  36. Kees UR, Heerema NA, Kumar R, et al. Expression of HOX11 in childhood T-lineage acute lymphoblastic leukaemia can occur in the absence of cytogenetic aberration at 10q24: a study from the Children's Cancer Group (CCG). Leukemia. 2003;17: 887-893.[CrossRef][Medline] [Order article via Infotrieve]

  37. Ferrando AA, Herblot S, Palomero T, et al. Biallelic transcriptional activation of oncogenic transcription factors in T-cell acute lymphoblastic leukemia. Blood. 2004;103: 1909-1911.[Abstract/Free Full Text]

  38. Alkema MJ, Wiegant J, Raap AK, Berns A, van Lohuizen M. Characterization and chromosomal localization of the human proto-oncogene BMI-1. Hum Mol Genet. 1993;2: 1597-1603.[Abstract/Free Full Text]

  39. Lessard J, Sauvageau G. Bmi-1 determines the proliferative capacity of normal and leukaemic stem cells. Nature. 2003;423: 255-260.[CrossRef][Medline] [Order article via Infotrieve]

  40. Hanson RD, Hess JL, Yu BD, et al. Mammalian Trithorax and polycomb-group homologues are antagonistic regulators of homeotic development. Proc Natl Acad Sci U S A. 1999;96: 14372-14377.[Abstract/Free Full Text]

  41. Nagel S, Kaufmann M, Drexler HG, MacLeod RA. The cardiac homeobox gene NKX2-5 is deregulated by juxtaposition with BCL11B in pediatric T-ALL cell lines via a novel t(5;14)(q35.1;q32.2). Cancer Res. 2003;63: 5329-5334.[Abstract/Free Full Text]

  42. Schneider NR, Carroll AJ, Shuster JJ, et al. New recurring cytogenetic abnormalities and association of blast cell karyotypes with prognosis in childhood T-cell acute lymphoblastic leukemia: a Pediatric Oncology Group report of 343 cases. Blood. 2000;96: 2543-2549.[Abstract/Free Full Text]

  43. Stern MH, Lipkowitz S, Aurias A, Griscelli C, Thomas G, Kirsch IR. Inversion of chromosome 7 in ataxia telangiectasia is generated by a rearrangement between T-cell receptor beta and T-cell receptor gamma genes. Blood. 1989;74: 2076-2080.[Abstract/Free Full Text]

  44. Bernard O, Groettrup M, Mugneret F, Berger R, Azogui O. Molecular analysis of T-cell receptor transcripts in a human T-cell leukemia bearing a t(1;14) and an inv(7); cell surface expression of a TCR-beta chain in the absence of alpha chain. Leukemia. 1993;7: 1645-1653.[Medline] [Order article via Infotrieve]

  45. Krumlauf R. Hox genes in vertebrate development. Cell. 1994;78: 191-201.[CrossRef][Medline] [Order article via Infotrieve]

  46. Kondo T, Duboule D. Breaking colinearity in the mouse HoxD complex. Cell. 1999;97: 407-417.[CrossRef][Medline] [Order article via Infotrieve]

  47. Brend T, Gilthorpe J, Summerbell D, Rigby PW. Multiple levels of transcriptional and posttranscriptional regulation are required to define the domain of Hoxb4 expression. Development. 2003;130: 2717-2728.[Abstract/Free Full Text]

  48. Spitz F, Gonzalez F, Duboule D. A global control region defines a chromosomal regulatory landscape containing the HoxD cluster. Cell. 2003;113: 405-417.[CrossRef][Medline] [Order article via Infotrieve]

  49. Whitehurst CE, Chattopadhyay S, Chen J. Control of V(D)J recombinational accessibility of the D beta 1 gene segment at the TCR beta locus by a germline promoter. Immunity. 1999;10: 313-322.[CrossRef][Medline] [Order article via Infotrieve]

  50. Mansfield JH, Harfe BD, Nissen R, et al. MicroRNA-responsive `sensor' transgenes uncover Hox-like and other developmentally regulated patterns of vertebrate microRNA expression. Nat Genet. 2004;36: 1079-1083.[CrossRef][Medline] [Order article via Infotrieve]

  51. Chambeyron S, Bickmore WA. Chromatin decondensation and nuclear reorganization of the HoxB locus upon induction of transcription. Genes Dev. 2004;18: 1119-1130.[Abstract/Free Full Text]

  52. Lowney P, Corral J, Detmer K, et al. A human Hox 1 homeobox gene exhibits myeloid-specific expression of alternative transcripts in human hematopoietic cells. Nucleic Acids Res. 1991;19: 3443-3449.[Abstract/Free Full Text]

  53. Milne TA, Briggs SD, Brock HW, et al. MLL targets SET domain methyltransferase activity to Hox gene promoters. Mol Cell. 2002;10: 1107-1117.[CrossRef][Medline] [Order article via Infotrieve]

  54. Nakamura T, Mori T, Tada S, et al. ALL-1 is a histone methyltransferase that assembles a supercomplex of proteins involved in transcriptional regulation. Mol Cell. 2002;10: 1119-1128.[CrossRef][Medline] [Order article via Infotrieve]

  55. Yokoyama A, Wang Z, Wysocka J, et al. Leukemia proto-oncoprotein MLL forms a SET1-like histone methyltransferase complex with menin to regulate Hox gene expression. Mol Cell Biol. 2004;24: 5639-5649.[Abstract/Free Full Text]

  56. Zeisig BB, Milne T, Garcia-Cuellar MP, et al. Hoxa9 and Meis1 are key targets for MLL-ENL-mediated cellular immortalization. Mol Cell Biol. 2004;24: 617-628.[Abstract/Free Full Text]

  57. Sauvageau G, Thorsteinsdottir U, Eaves CJ, et al. Overexpression of HOXB4 in hematopoietic cells causes the selective expansion of more primitive populations in vitro and in vivo. Genes Dev. 1995;9: 1753-1765.[Abstract/Free Full Text]

  58. Lawrence HJ, Sauvageau G, Humphries RK, Largman C. The role of HOX homeobox genes in normal and leukemic hematopoiesis. Stem Cells. 1996;14: 281-291.[Abstract]

  59. Izon DJ, Rozenfeld S, Fong ST, Komuves L, Largman C, Lawrence HJ. Loss of function of the homeobox gene Hoxa-9 perturbs early T-cell development and induces apoptosis in primitive thymocytes. Blood. 1998;92: 383-393.[Abstract/Free Full Text]

  60. So CW, Karsunky H, Wong P, Weissman IL, Cleary ML. Leukemic transformation of hematopoietic progenitors by MLL-GAS7 in the absence of Hoxa7 or Hoxa9. Blood. 2004;103: 3192-3199.[Abstract/Free Full Text]

  61. Nakamura T, Largaespada DA, Shaughnessy JD Jr, Jenkins NA, Copeland NG. Cooperative activation of Hoxa and Pbx1-related genes in murine myeloid leukaemias. Nat Genet. 1996;12: 149-153.[CrossRef][Medline] [Order article via Infotrieve]

  62. Thorsteinsdottir U, Sauvageau G, Hough MR, et al. Overexpression of HOXA10 in murine hematopoietic cells perturbs both myeloid and lymphoid differentiation and leads to acute myeloid leukemia. Mol Cell Biol. 1997;17: 495-505.[Abstract]

  63. Look AT. Oncogenic transcription factors in the human acute leukemias. Science. 1997;278: 1059-1064.[Abstract/Free Full Text]

  64. Lawrence HJ, Rozenfeld S, Cruz C, et al. Frequent co-expression of the HOXA9 and MEIS1 homeobox genes in human myeloid leukemias. Leukemia. 1999;13: 1993-1999.[CrossRef][Medline] [Order article via Infotrieve]

  65. Owens BM, Hawley RG. HOX and non-HOX homeobox genes in leukemic hematopoiesis. Stem Cells. 2002;20: 364-379.[Abstract/Free Full Text]

  66. Borrow J, Shearman AM, Stanton VP Jr, et al. The t(7;11)(p15;p15) translocation in acute myeloid leukaemia fuses the genes for nucleoporin NUP98 and class I homeoprotein HOXA9. Nat Genet. 1996;12: 159-167.[CrossRef][Medline] [Order article via Infotrieve]

  67. Nakamura T, Largaespada DA, Lee MP, et al. Fusion of the nucleoporin gene NUP98 to HOXA9 by the chromosome translocation t(7;11)(p15; p15) in human myeloid leukaemia. Nat Genet. 1996;12: 154-158.[CrossRef][Medline] [Order article via Infotrieve]

  68. Fujino T, Suzuki A, Ito Y, et al. Single-translocation and double-chimeric transcripts: detection of NUP98-HOXA9 in myeloid leukemias with HOXA11 or HOXA13 breaks of the chromosomal translocation t(7;11)(p15;p15). Blood. 2002;99: 1428-1433.[Abstract/Free Full Text]

  69. Ebert BL, Golub TR. Genomic approaches to hematologic malignancies. Blood. 2004;104: 923-932.[Abstract/Free Full Text]

  70. Chiaretti S, Li X, Gentleman R, et al. Gene expression profile of adult T-cell acute lymphocytic leukemia identifies distinct subsets of patients with different response to therapy and survival. Blood. 2004;103: 2771-2778.[Abstract/Free Full Text]

  71. Chervinsky DS, Zhao XF, Lam DH, Ellsworth M, Gross KW, Aplan PD. Disordered T-cell development and T-cell malignancies in SCL LMO1 double-transgenic mice: parallels with E2A-deficient mice. Mol Cell Biol. 1999;19: 5025-5035.[Abstract/Free Full Text]

  72. Herblot S, Steff AM, Hugo P, Aplan PD, Hoang T. SCL and LMO1 alter thymocyte differentiation: inhibition of E2A-HEB function and pre-T alpha chain expression. Nat Immunol. 2000;1: 138-144.[CrossRef][Medline] [Order article via Infotrieve]

  73. O'Neil J, Shank J, Cusson N, Murre C, Kelliher M. TAL1/SCL induces leukemia by inhibiting the transcriptional activity of E47/HEB. Cancer Cell. 2004;5: 587-596.[CrossRef][Medline] [Order article via Infotrieve]

  74. Lin WC, Desiderio S. Regulation of V(D)J recombination activator protein RAG-2 by phosphorylation. Science. 1993;260: 953-959.[Abstract/Free Full Text]

  75. Bellavia D, Campese AF, Checquolo S, et al. Combined expression of pTalpha and Notch3 in T cell leukemia identifies the requirement of preTCR for leukemogenesis. Proc Natl Acad Sci U S A. 2002;99: 3788-3793.[Abstract/Free Full Text]

  76. Bhatia-Gaur R, Donjacour AA, Sciavolino PJ, et al. Roles for Nkx3.1 in prostate development and cancer. Genes Dev. 1999;13: 966-977.[Abstract/Free Full Text]

  77. Bosher JM, Williams T, Hurst HC. The developmentally regulated transcription factor AP-2 is involved in c-erbB-2 overexpression in human mammary carcinoma. Proc Natl Acad Sci U S A. 1995;92: 744-747.[Abstract/Free Full Text]


Add to CiteULike CiteULike   Add to Connotea Connotea   Add to Del.icio.us Del.icio.us   Add to Digg Digg   Add to Reddit Reddit   Add to Technorati Technorati    What's this?


This article has been cited by other articles:


Home page
 BloodHome page
P. Van Vlierberghe, M. van Grotel, J. Tchinda, C. Lee, H. B. Beverloo, P. J. van der Spek, A. Stubbs, J. Cools, K. Nagata, M. Fornerod, et al.
The recurrent SET-NUP214 fusion as a new HOXA activation mechanism in pediatric T-cell acute lymphoblastic leukemia
Blood, May 1, 2008; 111(9): 4668 - 4680.
[Abstract] [Full Text] [PDF]

Home page
 haematolHome page
F. J.T. Staal and A. W. Langerak
Signaling pathways involved in the development of T-cell acute lymphoblastic leukemia
Haematologica, April 1, 2008; 93(4): 493 - 497.
[Full Text] [PDF]

Home page
 Clin. Cancer Res.Home page
F. Baleydier, A.-V. Decouvelaere, J. Bergeron, P. Gaulard, D. Canioni, Y. Bertrand, S. Lepretre, B. Petit, H. Dombret, K. Beldjord, et al.
T Cell Receptor Genotyping and HOXA/TLX1 Expression Define Three T Lymphoblastic Lymphoma Subsets which Might Affect Clinical Outcome
Clin. Cancer Res., February 1, 2008; 14(3): 692 - 700.
[Abstract] [Full Text] [PDF]

Home page
 BloodHome page
M. Fasseu, P. D. Aplan, M. Chopin, N. Boissel, J.-C. Bories, J. Soulier, H. von Boehmer, F. Sigaux, and A. Regnault
p16INK4A tumor suppressor gene expression and CD3{epsilon} deficiency but not pre-TCR deficiency inhibit TAL1-linked T-lineage leukemogenesis
Blood, October 1, 2007; 110(7): 2610 - 2619.
[Abstract] [Full Text] [PDF]

Home page
 BloodHome page
J. Bergeron, E. Clappier, I. Radford, A. Buzyn, C. Millien, G. Soler, P. Ballerini, X. Thomas, J. Soulier, H. Dombret, et al.
Prognostic and oncogenic relevance of TLX1/HOX11 expression level in T-ALLs
Blood, October 1, 2007; 110(7): 2324 - 2330.
[Abstract] [Full Text] [PDF]

Home page
 Cancer Res.Home page
D. Caudell, Z. Zhang, Y. J. Chung, and P. D. Aplan
Expression of a CALM-AF10 Fusion Gene Leads to Hoxa Cluster Overexpression and Acute Leukemia in Transgenic Mice
Cancer Res., September 1, 2007; 67(17): 8022 - 8031.
[Abstract] [Full Text] [PDF]

Home page
 BloodHome page
E. Clappier, W. Cuccuini, A. Kalota, A. Crinquette, J.-M. Cayuela, W. A. Dik, A. W. Langerak, B. Montpellier, B. Nadel, P. Walrafen, et al.
The C-MYB locus is involved in chromosomal translocation and genomic duplications in human T-cell acute leukemia (T-ALL), the translocation defining a new T-ALL subtype in very young children
Blood, August 15, 2007; 110(4): 1251 - 1261.
[Abstract] [Full Text] [PDF]

Home page
 BloodHome page
N. R. dos Santos, D. S. Rickman, A. de Reynies, F. Cormier, M. Williame, C. Blanchard, M.-H. Stern, and J. Ghysdael
Pre-TCR expression cooperates with TEL-JAK2 to transform immature thymocytes and induce T-cell leukemia
Blood, May 1, 2007; 109(9): 3972 - 3981.
[Abstract] [Full Text] [PDF]

Home page
 Proc. Natl. Acad. Sci. USAHome page
T. Palomero, W. K. Lim, D. T. Odom, M. L. Sulis, P. J. Real, A. Margolin, K. C. Barnes, J. O'Neil, D. Neuberg, A. P. Weng, et al.
NOTCH1 directly regulates c-MYC and activates a feed-forward-loop transcriptional network promoting leukemic cell growth
PNAS, November 28, 2006; 103(48): 18261 - 18266.
[Abstract] [Full Text] [PDF]

Home page
 BloodHome page
P. Van Vlierberghe, M. van Grotel, H. B. Beverloo, C. Lee, T. Helgason, J. Buijs-Gladdines, M. Passier, E. R. van Wering, A. J. P. Veerman, W. A. Kamps, et al.
The cryptic chromosomal deletion del(11)(p12p13) as a new activation mechanism of LMO2 in pediatric T-cell acute lymphoblastic leukemia
Blood, November 15, 2006; 108(10): 3520 - 3529.
[Abstract] [Full Text] [PDF]

Home page
 Proc. Natl. Acad. Sci. USAHome page
D. Bansal, C. Scholl, S. Frohling, E. McDowell, B. H. Lee, K. Dohner, P. Ernst, A. J. Davidson, G. Q. Daley, L. I. Zon, et al.
Cdx4 dysregulates Hox gene expression and generates acute myeloid leukemia alone and in cooperation with Meis1a in a murine model
PNAS, November 7, 2006; 103(45): 16924 - 16929.
[Abstract] [Full Text] [PDF]

Home page
 JCOHome page
C. D. Baldus, T. Burmeister, P. Martus, S. Schwartz, N. Gokbuget, C. D. Bloomfield, D. Hoelzer, E. Thiel, and W. K. Hofmann
High Expression of the ETS Transcription Factor ERG Predicts Adverse Outcome in Acute T-Lymphoblastic Leukemia in Adults
J. Clin. Oncol., October 10, 2006; 24(29): 4714 - 4720.
[Abstract] [Full Text] [PDF]

Home page
 Nucleic Acids ResHome page
C.-C. Liu, W.-S. E. Chen, C.-C. Lin, H.-C. Liu, H.-Y. Chen, P.-C. Yang, P.-C. Chang, and J. J.W. Chen
Topology-based cancer classification and related pathway mining using microarray data
Nucleic Acids Res., September 1, 2006; 34(14): 4069 - 4080.
[Abstract] [Full Text] [PDF]

Home page
 BloodHome page
J. L. Hess, C. B. Bittner, D. T. Zeisig, C. Bach, U. Fuchs, A. Borkhardt, J. Frampton, and R. K. Slany
c-Myb is an essential downstream target for homeobox-mediated transformation of hematopoietic cells
Blood, July 1, 2006; 108(1): 297 - 304.
[Abstract] [Full Text] [PDF]

Home page
 JCOHome page
S. A. Armstrong and A. T. Look
Molecular Genetics of Acute Lymphoblastic Leukemia
J. Clin. Oncol., September 10, 2005; 23(26): 6306 - 6315.
[Abstract] [Full Text] [PDF]

This Article
Right arrow Abstract Freely available
Right arrow Full Text (PDF)
Right arrow Supplemental Materials/Methods, Tables, and Figures
Right arrow All Versions of this Article:
2004-10-3900v1
106/1/274    most recent
Right arrow Alert me when this article is cited
Right arrow Alert me if a correction is posted
Right arrow Citation Map
Services
Right arrow Email this article to a friend
Right arrow Similar articles in this journal
Right arrow Similar articles in PubMed
Right arrow Alert me to new issues of the journal
Right arrow Download to citation manager
Right arrow reprints & permissions
Right arrow Rights and Permissions
Citing Articles
Right arrow Citing Articles via HighWire
Right arrow Citing Articles via CrossRef
Right arrow Citing Articles via Google Scholar
Google Scholar
Right arrow Articles by Soulier, J.
Right arrow Articles by Sigaux, F.
Right arrow Search for Related Content
PubMed
Right arrow PubMed Citation
Right arrow Articles by Soulier, J.
Right arrow Articles by Sigaux, F.
Related Collections
Right arrow Hematopoiesis and Stem Cells
Right arrow Neoplasia
Right arrow Gene Expression
Social Bookmarking
Add to CiteULike   Add to Connotea   Add to Del.icio.us   Add to Digg   Add to Reddit   Add to Technorati  
What's this?

click for free articles
home about blood authors subscriptions permissions advertising public access contact us
  Copyright © 2005 by American Society of Hematology         Online ISSN: 1528-0020