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(American Journal of Pathology. 2002;160:1487-1494.)
© 2002 American Society for Investigative Pathology

Regular Articles

Diversity of Genomic Breakpoints in TFG-ALK Translocations in Anaplastic Large Cell Lymphomas

Identification of a New TFG-ALK_XL Chimeric Gene with Transforming Activity

Luis Hernández^*, Sílvia Beà, Beatriz Bellosillo, Magda Pinyol, Brunangelo Falini, Antonino Carbone, German Ott^¶, Andreas Rosenwald^¶, Alberto Fernández^*, Karen Pulford^||, David Mason^||, Stephan W. Morris^**, Eugenio Santos^* and Elias Campo

From the Centro de Investigación delCáncer,^* Centro Superior de InvestigacionesCientíficas-University of Salamanca, Salamanca, Spain; theLaboratory of Pathology, Hospital Clinic,Institut d’Investigacions Biomediques August Pi i Sunyer, Universityof Barcelona, Barcelona, Spain; Institute ofHematology, Perugia University, Perugia,Italy; the Centro di Riferimento Oncologico, National Cancer Institute,Aviano, Aviano, Italy; the Institute ofPathology,^¶ University of Würzburg,Würzburg, Germany; the Leukemia Research FundImmunodiagnostics Unit,^|| Nuffield Department of ClinicalBiochemistry and Cellular Science, John Radcliffe Hospital, Oxford,United Kingdom; and the Departments of Pathology andHematology-Oncology,^** St. Jude Children’sResearch Hospital, Memphis, Tennessee

	Abstract

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Anaplastic large cell lymphomas are associated with chromosomal aberrations involving the anaplastic lymphoma kinase (ALK) gene at 2p23 that result in the expression of novel chimeric ALK proteins with transforming properties. In most of these tumors, the t(2;5)(p23;q35) generates the NPM-ALK fusion gene. However, several studies have now demonstrated that genes other than NPM may be fused to the ALK gene. We have recently described two different ALK rearrangements involving the TRK-fused gene (TFG) in which the same portion of ALK was fused to different length fragments of the 5' TFG region. These two rearrangements encoded chimeric proteins of 85 kd (TFG-ALK_S) and 97 kd (TFG-ALK_L), respectively. In this study, we have identified a new ALK rearrangement in which the catalytic domain of ALK was fused to a larger fragment of the TFG gene (TFG-ALK_XL), encoding for a fusion protein of 113 kd. Genomic analysis of these three TFG-ALK rearrangements revealed that the TFG breakpoints occur at introns 3, 4, and 5, respectively, whereas the ALK breakpoints always occur in the same intron. No homologous regions or known recombination sequences were found in these regions. Transfection experiments using NIH-3T3 fibroblasts showed a similar transforming efficiency of TFG-ALK variants compared with NPM-ALK. In addition, in common with NPM-ALK, the TFG-ALK proteins formed stable complexes with the signaling proteins Grb2, Shc, and PLC-. In conclusion, these findings indicate that the TFG may use a variety of intronic breakpoints in ALK rearrangements generating fusion proteins of different molecular weights, but with similar transforming potential than NPM-ALK.

The TFG gene at 3q11-12¹⁵ has been found to be a fusion partner of ALK in two cases of ALCL.⁹ Protein analysis of these tumors showed chimeric ALK proteins of 85-kd and 97-kd molecular weight, with a cytoplasmic-restricted localization. Molecular cDNA analysis of these cases showed that the TFG segment included in both translocations encoded the full predicted coiled-coil oligomerization domain of the protein. However, the chimeric gene coding for the 97-kd protein contained an additional 165-bp fragment of the TFG gene that was not included in the TFG-ALK gene coding for the 85-kd protein. Because of the different lengths of the chimeric products, these two fused genes were named TFG-ALK_S (short) and TFG-ALK_L (long), respectively. The larger TFG portion present in the TFG-ALK_L chimeric gene was the same as in the TFG-NTRK1 translocation that occurs in thyroid carcinomas.¹⁶ However, the genomic breakpoints of these translocations were not characterized.

In the present study, we examine the genomic breakpoints of the two previously described TFG-ALK rearrangements and identify a third TFG-ALK variant involving a new breakpoint located in TFG intron 5. We also demonstrate that TFG-ALK chimeric genes have in vitro transforming potential involving similar transduction pathway elements (Grb2, Shc, and PLC-) as the NPM-ALK gene.

	Materials and Methods

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Materials

The specimen used for the initial cloning studies was a diagnostic lymph node biopsy (case 893) from an 11-year-old female diagnosed with CD30-positive ALCL of null/T-cell phenotype (clinical stage IB) that was treated in 1991 according to the LSA2/L2 protocol and is at present in complete remission. ALK protein was expressed with a cytoplasmic-restricted pattern and a reverse transcriptase-polymerase chain reaction (RT-PCR) analysis was negative for the NPM-ALK fusion gene. Additional frozen material from the ALCLs with the two TFG-ALK fusion genes previously described (cases 789 and 862),⁹ were also used to determine the genomic breakpoint of these translocations.

Immunohistochemistry and Antibodies

Immunohistological staining of formalin-fixed paraffin-embedded tissues was performed using a panel of monoclonal antibodies for B- and T-cell antigens, together with antibodies to CD30 (DAKO-BerH2; DAKO, Copenhagen, Denmark) and EMA (DAKO-EMA/E29). Antibodies against the ALK protein (ALK1 and ALKc) and the N-terminal region of nucleophosmin used in the immunohistochemical and Western blot analyses were produced in the authors’ laboratories.^1,17,18 Immunohistochemical studies were also performed on NIH-3T3 fibroblasts transformed with NPM-ALK, TFG-ALK_S, and TFG-ALK_XL. Serial dilutions of these cells were seeded onto coverslips for 24 hours, washed twice with phosphate-buffered saline (PBS), then fixed with 95% ethanol/5% acetic acid at -20°C for 10 minutes. The cells were washed twice for 5 minutes each in PBS, and blocked with 10% heat-inactivated goat serum for 30 minutes at room temperature, then incubated overnight in a humidified chamber with polyclonal antibody ALK-11 (1:100 in 0.2% heat-inactivated goat serum/0.05% Triton X-100 PBS), washed again four times with PBS, then incubated for 45 minutes with a Cy3-conjugated affinity-purified goat anti-rabbit IgG secondary antibody (1:1000; Jackson ImmunoResearch Laboratories, Inc., West Grove, PA). The cells were washed again, and the nuclei counterstained with propidium iodide. The immunofluorescent staining was examined with an Axiovert 135 TV microscope and Hamamatsu XC77 digital camera.

RNA Extraction and RT-PCR of the TFG-ALK_XL Fusion Gene

Total RNA was isolated from a frozen sample of case 893 using the Ultraspec RNA extraction kit (Biotecx, Houston, TX), following the manufacturer’s recommendations. Reverse transcription was performed using Super Script II Reverse Transcriptase (Life Technologies, Inc., Paisley, UK) with random hexamer priming from 1 µg of total RNA. PCR amplification including the cDNA breakpoint region in case 893 was performed using the same TFG1 (5'-AGCTTGGAACCACCTGGAGAACC-3') and ALK3 (5'-GTCGAGGTGCGGAGCTTGCTCAGC-3') primers and reaction conditions described previously for the short and long TFG-ALK variants.⁹ The PCR product was purified and sequenced as previously described.⁹ RT-PCR analysis of other ALK fused genes (TPM-ALK, ATIC-ALK, and CLTC-ALK) was also performed using previously described primers.^8,10,14

Characterization of the Genomic Breakpoints in TFG-ALK Variants

Genomic DNA from the three tumors with different variants of the TFG-ALK fusion gene was prepared using Proteinase K treatment and phenol-chloroform extraction.¹⁹ Amplification of the genomic breakpoints was performed using a forward primer of the flanking TFG exon together with a common reverse ALK3 primer. TFG primers used were TFG1 for TFG-ALK_S and TFGLU (5'-GCAGCAAGTATGTCTGCTTTTGATCC-3') for TFG-ALK_L. Different TFG primers from the flanking exon and intronic region were designed to amplify the TFG-ALK_XL genomic breakpoint but all of these amplifications were unsuccessful. Amplification conditions were 40 cycles consisting of 45 seconds at 94°C, 45 seconds at 65°C, and 1 minute 30 seconds at 72°C. The PCR mixture contained 1 U of Taq polymerase (Boehringer Mannheim, Mannheim, Germany), 0.8 mmol/L of each primer, 100 mmol/L dNTPs, and PCR buffer in a final volume of 25 µl. Normal TFG introns involved in the TFG-ALK rearrangements were amplified using Pfx polymerase (Life Technologies, Inc.), and following the manufacturer’s specifications. The primers used were forward TGEN1U (5'-TGGGTGATTCTTTCGCAACTAGTC-3') and reverse TFG128D (5'CTGATCATCTGTTAAGCCAAACGC-3') for the normal TFG intron involved in the short variant, and forward TGEN9U (5'-GCTCTCCCAGCCCTATAGTCAG-3') and reverse XLDGENR (5'-AGGAGGAGGAAGCAATGCTGTC-3') for the normal TFG intron involved in the long variant. PCR products were purified and sequenced as previously described,⁹ using different upstream and downstream primers for primer walking. The computer program CENSOR, designed by Jurka and colleagues²⁰ was used by E-mail procedure (censor@charon.lpi.org) for repeat sequence identification. Other sequence features that were searched included interchromosomal homologies and positions of candidate recombination sequences (topoisomerase I and II, translin, heptamer/nonamer, chi consensus, alternating purine/pyrimidine, polypurine, and polypyrimidine sequences).^21-28

cDNA Cloning and DNA Constructs of the ALK Fusion Genes

TFG-ALK_XL, TFG-ALK_S, and NPM-ALK constructs were prepared by PCR-based methods and were expressed with the pMEX and pLTR2 plasmids.²⁹ The PsralphaMSVtkneo-NPM-ALK plasmid (trimmed of most of its 5' and 3' UTR sequences) was previously described.⁷ The NPM-ALK insert was released with HindIII and XbaI restriction enzymes, and then subcloned into the pMEX plasmid between EcoRI and SalI, and also subcloned into the pLTR2 plasmid between XhoI and ClaI sites. The TFG-ALK short and extra long cDNAs were cloned into the pMEX between XhoI and SalI restriction enzyme sites and also into the pLTR2 plasmid between XhoI and ClaI sites.

Focus Formation Assay

Mouse NIH-3T3 fibroblasts were maintained in Dulbecco’s modified Eagle’s medium (Life Technologies, Inc.) supplemented with 10% calf serum. Cells were seeded onto plastic dishes (1.5 x 10⁵ cells per dish) and transfected by the calcium-phosphate precipitation method as previously described,³⁰ using 0.2 to 2 µg of plasmid DNA (NPM-ALK, TFG-ALK_S, TFG-ALK_XL) together with 40 µg of high-molecular weight calf thymus carrier DNA. Each transfection was done in duplicate, and carrier DNA and empty plasmids were used as negative controls. H-RasK12 cloned into the pLTR2 was used as positive control. Transformed foci were selected in Dulbecco’s modified Eagle’s medium containing 5% calf serum and G418-resistant colonies were selected in Dulbecco’s modified Eagle’s medium supplemented with 10% serum and G418 antibiotic (750 µg/ml). Transformed foci and drug-resistant colonies were either stained with Giemsa solution or isolated for further studies 2 or 3 weeks after transfection.

Western Blot Analysis

Protein was extracted from cryostat frozen sections using a previously described method.³¹ Protein was also extracted from cells using a lysis buffer composed of 20 mmol/L HEPES, pH 7.5, 10 mmol/L EGTA, 40 mmol/L ß-glycerophosphate, 1% Nonidet P-40, 25 mmol/L MgCl₂, 2 mmol/L sodium orthovanadate, 2 mmol/L dithiothreitol, 1 mmol/L phenylmethyl sulfonyl fluoride, 10 µg/ml aprotinin, and 10 µg/ml leupeptin. Equal amounts of protein were separated by electrophoresis on SDS-10% polyacrylamide gels and transferred to Immobilon-P (Millipore, Bedford, MA) membranes. The membranes were incubated with monoclonal antibodies against ALK (ALK-1 and ALKc) or anti-NPM. Antibody binding was detected using a secondary antibody (anti-rabbit or anti-mouse immunoglobulin; Amersham, Buckinghamshire, UK) conjugated to horseradish peroxidase and an enhanced chemiluminescence detection kit (Amersham).

Immunoprecipitations

Cell lysates (1 mg) were incubated overnight with 10 µl of antibodies to one of the following: ALK, Shc (Transduction Laboratories, Lexington, KY), Grb2 (Transduction Laboratories), or PLC- (Santa Cruz Biotechnology, Inc., Santa Cruz, CA) antibodies at 4°C. Protein A-Sepharose was then added to the samples for 1 hour at 4°C. Immunoprecipitates were washed three times with lysis buffer and electrophoresed in 10 to 20% polyacrylamide gradient gels (Bio-Rad). The proteins were then transferred to Immobilon-P and detected using anti-ALK as described above.

	Results

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Characterization of the TFG-ALK_XL Variant

The lymph node biopsy of case 893 showed a typical ALCL of common morphology expressing CD30 and epithelial membrane antigen. ALK protein was detected in all tumor cells and exhibited a cytoplasmic-restricted expression pattern. Immunohistochemical staining using monoclonal antibodies against the N-terminal portion of NPM detected only nuclear NPM protein. Western blot analysis using anti-ALK and anti-NPM (N-terminus) antibodies detected an abnormal ALK protein with an apparent molecular weight of 113 kd, and only the wild-type 38-kd NPM protein (Figure 1) . These findings indicated that a partner other than NPM was fused to ALK in this tumor.³²

View larger version (41K): [in this window] [in a new window]   Figure 1. Western blotting of protein extracted from sections of the anaplastic large-cell lymphoma 893 using anti-ALKc demonstrates the presence of a 113-kd TFG-ALKXL fusion protein in tumor cells.

View larger version (74K): [in this window] [in a new window]   Figure 2. A: PCR amplification of the cDNA breakpoint region using primers from the TFG and ALK genes. Cases with the TFG-ALK S, L, and XL variants showed amplification products of different sizes (141, 306, and 447 bp, respectively). C- represents the negative PCR control without template. B: Nucleotide and amino acid sequence of the TFG-ALKXL cDNA junction. Underlined sequence corresponds to the 141 bp of TFG exon 5 present only in the TFG-ALKXL variant. The translocation breakpoint in the cDNA is marked with an arrow. C: Automated sequence profile of the breakpoint region in the TFG-ALKXL variant.

The TFG-ALK_XL genomic breakpoint could not be amplified despite the use of numerous different primers. Nevertheless, the human TFG genomic organization could be obtained from alignment analysis of the TFG cDNA sequence with the corresponding genomic sequence of human chromosome 3 (GenBank accession NT_005863). This information revealed that the extra sequence of TFG present in the cDNA of the TFG-ALK_XL variant corresponded to a complete exon 5; thus, the genomic breakpoint in this case must be located within TFG intron 5 (Figure 3) . Considering the size of the introns involved in this rearrangement (8116 bp for TFG and 1935 bp for ALK), the rearranged intron of the resulting TFG-ALK_XL fusion gene may be around 10 kb long, helping to explain our difficulty in amplifying this fragment.

View larger version (16K): [in this window] [in a new window]   Figure 3. Genomic organization of TFG-ALKS, TFG-ALKL, and TFG-ALKXL variants. Intronic organization is detailed only for the TFG sequence. The striped box in the ALK sequence represents the kinase domain.

Several possible mechanisms leading to the genomic breakpoints involving TFG and ALK were explored by analyzing for the presence of homologous regions and candidate recombination sequences. However, no significant homologous, repeated, or consensus sequences were found in the involved intronic regions (all of the homologies found scored below 50%).

Oncogenic Potential of TFG-ALK Fusion Transcripts

To assess the oncogenic activity of the TFG-ALK variants, we cloned the full-length TFG-ALK_S and TFG-ALK_XL cDNAs into the pMex and pLTR2 expression vectors. These constructs were transfected into NIH-3T3 fibroblasts and the transforming activity was analyzed in focus formation assays. Cells transfected with NPM-ALK, TFG-ALK_S, and TFG-ALK_XL produced similar numbers of foci/µg of cDNA, with slightly higher transforming efficiency observed for TFG-ALK_S. No foci were observed after transfection with empty vectors or carrier DNA (Table 1) . Cells picked from the foci showed the typical morphology and lack of contact inhibition of transformed cells.

Association of ALK Fusion Proteins with Grb2, Shc, and PLC-

We next analyzed whether these TFG-ALK fusion proteins had similar activation mechanisms to those that have been previously described for the NPM-ALK and ATIC-ALK fusion proteins. Cell lysates from NIH-3T3 clones expressing NPM-ALK, TFG-ALK_S, or TFG-ALK_XL were immunoprecipitated with anti-Shc, anti-Grb2, and anti-PLC- antibodies, then blotted with anti-ALK antibody. As seen in Figure 4 , TFG-ALK_S was co-immunoprecipitated with Shc, Grb2, and PLC-, indicating an interaction between these proteins. Similar results were observed with TFG-ALK_XL, although a slightly smaller amount of this protein was co-immunoprecipitated with Grb2. These results indicate that TFG-ALK fusion proteins are associated in cells with the same signaling intermediates used by NPM-ALK for signal transduction, suggesting that different ALK chimeric products likely use similar transforming pathways.

View larger version (57K): [in this window] [in a new window]   Figure 4. Interaction of TFG-ALK variants with PLC-, Grb2, and Shc. Cell lysates from NIH-3T3 clones expressing NPM-ALK, TFG-ALKS, or TFG-ALKXL were immunoprecipitated with the indicated antibodies, then analyzed by Western blot using anti-ALK. IP, immunoprecipitated; SN, supernatant.

	Discussion

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In the present work we described three different TFG intronic breakpoints involving in all of the cases a rearrangement with the ALK gene, thus indicating that the TFG gene structure may facilitate multiple rearrangements with different genomic sequences. This diversity in the number of breakpoints may be because in part of the fact that the three TFG intronic regions described in this work and an additional 3' intron of TFG may fuse with ALK generating in-frame transcripts that also maintain the oligomerization domain of the protein. On the contrary, NPM, TPM3, and CLTC genes have only one possible intron that would allow a rearrangement with ALK resulting in an in-frame sequence including the oligomerization domain of the partner. The other two ALK fused genes, MSN and ATIC, have two and three potential introns, respectively, that may fuse in-frame with ALK, but, so far only one type of chimeric gene has been described.

The sequence retained in all of the TFG translocations contained the predicted coiled-coil oligomerization domain of the protein, a region that, like the dimerization motif of NPM in the NPM-ALK fusion, is absolutely required for oligomerization and the transforming activity of the TFG-NTRK (TRK-T3) oncoprotein.³³ Therefore, it is also likely that TFG plays a similar role in the activation of ALK in ALCL. However, in contrast to NPM, TFG lacks nuclear localization-signaling domains, a finding that is in keeping not only with the cytoplasmic-only pattern of ALK expression observed in our immunohistochemical analysis of the three variants in ALCL specimens, but also with the immunocytochemical localization of the TFG-ALK_S and TFG-ALK_XL fusion proteins in NIH-3T3-transformed cells.

Recurrent chromosome translocations are characteristic of a number of human hematological tumors. It has been proposed that homologous recombination and/or site-specific recombinogenic sequences may be implicated in the generation of these reciprocal translocations. The lymphoid-specific recombinogenic machinery could be involved in some translocation events through heptamer/nonamer or translin consensus sequences. In addition, other types of promoting sequences have been suggested to play a role in several translocations by using different recombinogenic mechanisms. Among these, topoisomerase I and II, chi consensus, Alu, palindromic, purine/pyrimidine, polypurine, or polypyrimidine sequences have been suggested as potential sequences involved in translocations.^21-28 In the present work, we have analyzed the genomic organization and intronic sequences of ALK translocations involving TFG. Only poor homologies with previously described recombinogenic sequences were found in the genomic regions surrounding the translocation breakpoints in both the TFG-ALK_S and TFG-ALK_L chimeric genes. Alternatively, an illegitimate recombination process may be involved in these translocations. This mechanism has been proposed for translocations occurring in different tumors and involves an independent generation of single strand DNA ends that are processed individually before interchromosomal joining.³⁴ This process frequently results in local sequence duplications, deletions, or inversions in the rearranged flanking sequences.³⁴ In keeping with this, we have recently described the MSN-ALK translocation to be associated with a 66-bp deletion in the derivative chromosome.¹³ However, these features were not found in the short and long TFG-ALK rearrangements described here, although the inserted thymidine found in the TFG-ALK_L variant could be interpreted as a duplication of an upstream ALK thymidine close to the breakpoint. Unfortunately, the amplification of the derivative chromosome 2 translocation was unsuccessful in both cases; thus, the presence of duplications, deletions, or inversions in these resulting regions could not be assessed. Recently, it was described that the illegitimate recombination process might be promoted by the proximity of the involved sequences in the nucleus.³⁵ It would be interesting to know the possible contribution of this mechanism to the generation of ALK translocations with its different partners.

The transforming potential of the NPM-ALK fusion gene has been previously demonstrated in in vitro experiments using rodent fibroblasts and in vivo in a murine model using retroviral transduction of bone marrow.^7,36,37 Downstream targets of the resulting constitutive ALK tyrosine kinase activation by the NPM-ALK fusion protein have been characterized in different studies and include proliferation-related elements such as Shc, Grb2, PLC-, IRS-1, and STAT5,^36,38-40 as well as the PI3K p85 subunit and PKB/AKT that result in an inhibition of apoptosis.^38,40,41 However, whether all these mediators play a role in the pathogenesis of ALCL is not clear because experiments using NPM-ALK mutants suggest that neither IRS-1 nor Shc are essential for transformation.^7,36 The possible transforming potential and signaling pathways of other ALK fusion proteins are not well known. In the ATIC-ALK variant, transformation potential was demonstrated in vitro using NIH-3T3 fibroblasts and the murine pro-B cell line BaF3.^11,12 Similar to NPM-ALK, the ATIC-ALK protein seems also to form stable complexes with Grb2 and Shc. In the present work, the transforming activity of TFG-ALK_S and TFG-ALK_XL could be analyzed in vitro, showing a transformation potential similar to NPM-ALK and also the binding with Grb2, Shc, and PLC-.

In conclusion, we have characterized a third variant of the TFG-ALK rearrangements (TFG-ALK_XL) involving TFG intron 5 and the same ALK intron found in other ALK translocations. This finding and the identification of TFG genomic breakpoints in introns 3 and 4 in previous TFG-ALK variants confirm the peculiar versatility of TFG as an activating partner in oncogenic translocations. We also demonstrate that TFG-ALK chimeric proteins have in vitro transforming potential and bind to some of the molecules that are also associated with the NPM-ALK fusion protein.

	Footnotes

 
Address reprint requests to Elias Campo, Laboratory of Pathology, Hospital Clinic, Villarroel 170, 08036, Barcelona, Spain. E-mail: campo{at}medicina.ub.es

Supported by the Spanish Comision Interministerial de Ciencia y Tecnologia (SAF 99/20 and FEDER 1FD97-1678), Associazione Italiana per la Ricerca sul Cancro (AIRC) the National Cancer Institute (grant CA69129 to S. W. M., CORE grant CA21765), and by the American Lebanese Syrian Associated Charities, St. Jude Children’s Research Hospital.

Genbank accession numbers for the genomic breakpoints of TFG-ALK_S, TFG-ALK_L and the TFG-ALK_XL cDNA are AF390891, AF390892, and AF390893, respectively.

Accepted for publication December 20, 2001.

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