Fusion of ETV6 to Neurotrophin-3 Receptor TRKC in Acute Myeloid Leukemia With t(12;15)(p13;q25)

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Blood, Vol. 93 No. 4 (February 15), 1999: pp. 1355-1363
Fusion of ETV6 to Neurotrophin-3 Receptor TRKC in Acute Myeloid Leukemia With t(12;15)(p13;q25)

By Mariko Eguchi, Minenori Eguchi-Ishimae, Arinobu Tojo, Kazuhiro Morishita, Katsuyuki Suzuki, Yuko Sato, Shiori Kudoh, Kimio Tanaka, Misao Setoyama, Fumitaka Nagamura, Shigetaka Asano, and Nanao Kamada
From the Department of Cancer Cytogenetics and the Department of Biochemistry and Biophysics, Research Institute for Radiation Biology and Medicine, Hiroshima University, Hiroshima, Japan; the Department of Hematology/Oncology, Institute of Medical Science, University of Tokyo, Tokyo, Japan; the Biology Division, National Cancer Center Research Institute, Tokyo, Japan; and the Division of Intractable Disease, Research Institute, International Medical Center of Japan, Tokyo, Japan.

  ABSTRACT

Top
Abstract
Introduction
References

Chromosome translocations involving band 12p13 are known to be involved in a variety of hematologic malignancies, some ofthem resulting in rearrangement of the ETV6/TEL gene. Applyingthe fluorescence in situ hybridization (FISH) method, we founda cryptic translocation t(12;15)(p13;q25) in an adult acute myeloidleukemia (AML) patient. Hybridization with cosmid probes showedthat the ETV6 gene was rearranged in this translocation. A patient-specificcDNA library was screened with ETV6 cDNA, and a novel fusion transcriptwas identified between the ETV6 and TRKC/NTRK3 gene located on15q25. TRKC is a receptor tyrosine kinase that is activated byneurotrophin-3 (NT-3). It is known to be expressed broadly inneural tissues but not in hematologic cells, so far. ETV6-TRKCchimeric transcript encoded the pointed (PNT) domain of the ETV6gene that fused to the protein-tyrosine kinase (PTK) domain ofthe TRKC gene. Two types of fusion transcript were determined,one that included the entire PTK domain of TRKC and the otherin which the 3'-terminal 462 bp of TRKC was truncated within thePTK domain. Western blot analysis showed the expression of bothchimeric proteins of 52 and 38 kD in size. Our results suggestthat chimeric PTK expressed in the leukemic cells may contributeto cellular transformation by abnormally activating TRK signalingpathways. Moreover, this is the first report on truncated neurotrophinreceptors associated inleukemia.
© 1999 by The American Society of Hematology.

  INTRODUCTION

Top
Abstract
Introduction
References

SPECIFIC CHROMOSOME abnormalities found in hematologic and nonhematologic malignancies have given many important insightsinto the pathogenesis of malignant transformation. Recent molecularbiological studies have shown that important genes associatedwith cell proliferation and/or differentiation are often involved.¹Cytogenetic abnormalities involving the short arm of chromosome12 have been observed in a wide variety of hematologic malignancies,including acute myeloid leukemia (AML), acute lymphoid leukemia(ALL), and myelodysplastic syndrome (MDS). The ETV6/TEL gene,cloned from chronic myelomonocytic leukemia harboring t(5;12)(q33;p13)as the translocation partner of platelet-derived growth factorreceptor $beta$ (PDGFR $beta$ ),² is now known to be disrupted in someof these 12p13 abnormalities.³ ETV6 is a member of the ETSfamily of transcriptional regulators that are defined by the ETSdomain responsible for specific DNA binding activities. It isalso distinctive in having the pointed (PNT) domain (also referredto as helix-loop-helix oligomerization domain) that is suggestedto play a role in the protein-protein interaction of ETS factors.²Besides t(5;12), the ETV6 gene is reported to form fusion transcriptsin some other 12p13-associated translocations, ie, ETV6-JAK2 inmyeloproliferative disorders (MPD) or ALL with t(9;12)(p24;p13)⁴^,⁵;ETV6-MN1 in MPD with t(12;22)(p13;q11)⁶; ETV6-MDS1/EVI1 inMPD with t(3;12)(q26;p13)⁷; and ETV6-AML1,⁸^,⁹ ETV6-ABL,¹⁰^,¹¹and ETV6-STL¹² in childhood B-precursor ALL with t(12;21)(p13;q22),t(9;12)(q34;p13), or t(6;12)(q23;p13),respectively.

Several members of the ETS family are known to be associated with various malignancies as the result of specific chromosometranslocations. These include t(11;22)(q24;q12) and t(7;22)(p22;q12)in Ewing's sarcoma¹³^,¹⁴ and t(21;22)(q22;q12) in clear cellsarcoma.¹⁵ In these translocations, the transactivation motifof EWS fuses to the ETS binding motif of FLI1, ETV1, or ERG, respectively,which are suspected to be oncogenic. In contrast to these EWS-associatedtranslocations, the ETV6 fusion gene mentioned above, with exceptionof ETV6-MN1 and ETV6-STL, loses its ETS binding domain but retainsthe PNT domain in the 5' ETV6 fusion transcript, indicating somedifferent underlying mechanism intransformation.

Translocation involving ETV6 is often subtle and therefore overlooked by conventional cytogenetic analysis. We report herea novel ETV6-associated translocation, t(12;15)(p13;q25), detectedby fluorescence in situ hybridization (FISH) analysis in an adultAML patient. A patient-specific cDNA library was screened withETV6 cDNA, and a fusion transcript between the ETV6 and TRKC/NTRK3gene was identified. The fusion transcript encoded the PNT domainof ETV6 that fused to the protein-tyrosine kinase (PTK) domainof TRKC. Abnormal protein expression was detected by Western blotanalysis, which was suspected to beoncogenic.

  MATERIALS AND METHODS

Patient material. Bone marrow samples obtained from a 59-year-old AML (FAB M2) patient with chromosome abnormalities of 48,XX,add(6)(q27),+8,inv(12)(p13q15),add(15)(q25),+add(15)(q25) were used in this study.The clinical and cytogenetic data of the patient have been describedpreviously.¹⁶ Despite aggressive chemotherapy, she died of multipleorgan failure associated with massive infiltration of leukemiccells in the systemic organs, 5 months after the onset of theleukemia.

Cytogenetic studies. The metaphase samples were prepared from bone marrow cells, which were fixed after unstimulated short-term cultures. G-bandedkaryotypes were determined according to the International Systemfor Human Cytogenetic Nomenclature (ISCN 1995¹⁷).

FISH analysis. Metaphase sample that was applied to cytogenetic studies was also used for FISH analysis. Probes used were 964c10 YAC probecovering the ETV6 locus on chromosome 12p13 (kindly provided byDr Janet D. Rowley, Section of Hematology/Oncology, Universityof Chicago, Chicago, IL³), LL12NCO1 cosmid probes (179A6, 163E7,and 148B6, which are located within the ETV6 gene; kindly providedby Dr Peter Marynen, Center for Human Genetics, Flanders InteruniversityInstitute for Biotechnology, Leuven, Belgium¹⁸), c-FES genomicprobe (provided by HSRRB, Osaka, Japan), 170I1 BAC clone locatedon 15q25 (Research Genetics, Huntsville, AL), and D12Z3 (Oncor,Gaithersburg, MD), which hybridizes to the $alpha$ satellite regionof chromosome 12. The probes were labeled with biotin-11-dUTPor digoxigenin-11-dUTP (Boehringer Mannheim, Mannheim, Germany)using polymerase chain reaction (PCR) labeling after sequence-independentamplification,¹⁹ and were hybridized to metaphase samples aspreviously described.²⁰ The probes were detected with avidinfluorescein (Vector Laboratories, Burlingame, CA) or anti-digoxigeninrhodamine (Boehringer Mannheim) and then counterstained with 4'6-diamidino-2-phenylindole dihydrochloride (DAPI). Images of thehybridized signals were captured under fluorescence microscopy(Olympus Optical Co, Tokyo,Japan).

Molecular cloning of the fusion mRNA. Poly(A)+ RNA was extracted from leukemic cells with a Fast Track mRNA Isolation Kit (Invitrogen, San Diego, CA). Five microgramsof the extracted mRNA was reverse transcribed using cDNA synthesismodule by random hexamer (Amersham, Buckinghamshire, UK), ligatedwith EcoRI-Not I-BamHI adaptor (Takara, Kyoto, Japan), and subclonedinto EcoRI-digested $lambda$ Zap II vector (Stratagene, La Jolla, CA).The constructed cDNA library was screened with ETV6 full-lengthcDNA (kindly provided by Dr Todd R. Golub, Division of PediatricOncology, Dana-Farber Cancer Institute, Boston, MA²). The positiveclones were isolated and subcloned into pBluescript phagemidsaccording to the manufacturer's instructions. Nucleotide sequenceswere determined using fluorescently labeled dideoxy terminatorson 373A Applied Biosystems automated sequencer (Applied Biosystems,Urayasu, Japan). The sequence of nucleotides was compared withthose in databases on the NCBI Blast server (Bethesda,MD).

Northern blot analysis. Total RNA of the leukemic cells was isolated by the acid guanidinium thiocyanate-phenol-chloroform method. Ten microgramsof the RNA was separated by electrophoresis on 1.2% agarose gelscontaining 0.7 mol/L formaldehyde and transferred to Hybond-Nmembranes (Amersham). Probes used for hybridization were full-lengthETV6 cDNA and TRKC cDNA fragment (at nucleotide position [nt]1556-1970²¹) prepared by PCR from fetal brain cDNA library (Clontech,Palo Alto, CA). Primers used were TRKC-1556f (5'-CGTGGCTGTCATCAGTGGTGAGG-3')and TRKC-1947r (5'-CCATAGAACTTGACAATGTGCTC-3'). The same filterwas rehybridized with a $beta$ -actin-specific probe to check the amountof RNA loaded in eachlane.

Reverse transcriptase-mediated PCR (RT-PCR). One microgram of the total RNA was reverse transcribed with 10 U of Moloney murine leukemia virus reverse trancriptase (MMLV-RT;Stratagene) using a random hexamer. One tenth of the synthesizedcDNA was directed to PCR analysis using a PCR kit (Takara). ThePCR conditions were as follows: 94°C for 3 minutes, followed by30 cycles of 94°C for 1 minute, 55°C for 1 minute, 72°C for 1minute and, finally, extension at 72°C for 10 minutes. The productswere electrophoresed on 3% agarose gels and stained by ethidiumbromide. The primers used were ETV6-116f (5'-CGATTCCGCCACTTCATGTTCCA-3'),ETV6-575r (5'-CGGTGATTTGTCGTGATAGGTG-3'), and TRKC primers mentionedabove. Total RNA extracted from NBTM cell line, which was derivedfrom a neuroblastoma (kindly provided by Dr Akira Nakagawara,Division of Biochemistry, Chiba Cancer Center, Chiba, Japan),was used as the positive control for TRKCexpression.

Anchored PCR analysis. Poly(A)+ RNA was extracted from the leukemic cells, and 500 ng was reverse transcribed and ligated with EcoRI-Not I-BamHIadaptor as mentioned above. To detect the 3' ETV6 mRNA, PCR analysiswas performed with adaptor primer (5'-AATTCGGCGGCCGCGGATCC-3')as the sense primer and ETV6-541rE (5'-CGAATTCGCAACAGTTCAATGGTGGGAGG-3')as the antisense primer. To detect the 5' TRKC mRNA, PCR was performedwith TRKC-1602fE (5'-CGAATTCCACATCAACCACGGCATCACC-3') as the senseprimer and adaptor primer as the antisense primer. The PCR conditionswere the same as previously described. The resulting PCR productwas subcloned into EcoRI/BamHI-digested into pBluescript phagemid(Stratagene) andsequenced.

Western blot analysis. Leukemic cells (2 × 10⁷) were washed in PBS; suspended in RIPA that contained 1% NP-40, 0.5% deoxycholate, and 0.5 mmol/L phenylmethylsulfonyl fluoride (PMSF); homogenized with a Dounce homogenizer;and kept on ice for 30 minutes. The samples were centrifuged at12,000g to remove any insoluble particles. Twenty-five microgramsof protein was separated on 10% sodium dodecyl sulfate (SDS)-polyacrylamidegels and transblotted onto Hybond-ECL membranes (Amersham). Afterappropriate blocking with 5% bovine serum albumin (BSA; SigmaCo, St Louis, MO), immunoblot analysis was performed with anti-TRK(C-14; Santa Cruz Biotechnology, Santa Cruz, CA), anti-N-TEL (kindlyprovided by Dr Olivier Bernard, U434 INSERM, Paris, France), andanti- $beta$ -actin antibodies (Santa Cruz). The signal was detectedby incubating with horseradish peroxidase (HRP)-conjugated secondantibody according to the manufacturer's instructions and wasexposed on FUJI RX film (FUJI Photo Film, Tokyo,Japan).

  RESULTS

Rearrangement of the ETV6 gene in complex translocations between 12p13, 12q15, and 15q25. To know whether the ETV6 gene was involved in inv(12)(p13q15), we applied FISH analysis using the 964c10 YAC probe that coversthe ETV6 gene. The signals turned out to be located on normal12p13, on der(12)(q15), and on two der(15)(q25), but not on der(12)(p13)(Fig 1A and B).¹⁶ This result caused us to hybridize the metaphasewith cosmid probes (179A6, 163E7, and 148B6) that locate withinthe ETV6 gene. As a result, 179A6 hybridized on two der(15)(q25),148B6 on der(12)(q15), and 163E7, which spans exon 3 to exon 5of the ETV6 gene, was detected as split signals between der(12)(q15)and two der(15)(q25) (Figs 1A and B and 2A). These results indicatedthat two events, t(12;15)(p13;q25) and inv(12)(p13q15), occurredwithin the ETV6 gene in the leukemic cells.

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Fig 1. (A) Physical map surrounding ETV6. The cosmid and YAC probes used in FISH analysis are shown underneath. (B) Schematic representation of t(12;15)(p13;q25) and inv(12)(p13q15) detected in the leukemic cells. Circles on the right indicate localization of probes detected in FISH analysis.

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Fig 2. FISH analysis of ETV6 and TRKC gene rearranged in the metaphase chromosomes. (A) Split signals of cosmid 163E7 (red) are observed on der(12)(q15) and on der(15)(q25). Large arrow indicates der(12), which is identified by chromosome 12 centromeric probe (D12Z3; green). The small arrows indicate der(15). Note that two der(15)s are detected in most metaphases. Large arrowhead indicates normal chromosome 12. (B) 170I1 BAC probe hybridized with 964c10 YAC probe. The 170I1 BAC (red) that encompasses the breakpoint of TRKC shows split signals on der(15)(q25) and on der(12)(p13). 964c10 YAC (green) covering ETV6 locus splits between der(12)(q15) and der(15)(q25), which results in fusion with 170I1 BAC signal on der(15)(q25). Normal chromosome 15 is indicated by a small arrowhead.

Cloning and identification of a novel ETV6 fusion product. To identify the fusion partner of the ETV6 gene, we constructed a cDNA library from leukemic cells that consisted of 1.25× 10⁵ independent clones and was screened with the full-length ETV6cDNA probe. Five positive clones were obtained and were subclonedin pBluescript phagemid. Sequence analysis showed that two clonesincluded a full-length ETV6 sequence, and the other three clonesincluded ETV6 exon 1 to exon 4, followed by an unknown sequence,which was proven to be TRKC by BLAST database searching (ETV6was referred to GenBank accession no. U11732 and human TRKCto U05012). In one clone (C-1), 487 bp of the ETV6 sequence,including the entire PNT domain, fused in-frame to the 3'-terminal1,010 bp of the human TRKC gene. The fusion point of ETV6 wasafter nt 487, which is the end of exon 4, followed by nt 1741of TRKC, including the entire PTK domain of TRKC (Fig 3). In theother two clones (C-2 and C-3), 487 bp of ETV6 fused to TRKC nt1741 just the same as the C-1 clone, but the 3'-terminal 462 bpof TRKC was truncated at TRKC nt 2288 within the PTK domain, followedby 2 unrelated amino acids and a TGA stop codon (see Fig 7). Thisunreported sequence after TRKC nt 2288 was confirmed to originatein the read-through intron sequence of normal TRKC by PCR forgenomic DNA (data not shown). This short-form TRKC mRNA seemsto be one of the splice variants of TRKC, because it is detectedby RT-PCR in neuroblastoma samples that express TRKC (data notshown). Sequence analysis showed a deduced 450 amino acid openreading frame in C-1 that was suspected to code 52-kD protein,and a 339 amino acid open reading frame in C-2 and C-3 that weresuspected to code 38-kD protein. The cDNA library was rehybridizedwith the TRKC cDNA probe spanning the breakpoint, but no positiveclone including the 5'-portion of TRKC was obtained.

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Fig 3. Schematic representation of ETV6, TRKC, and predicted ETV6-TRKC protein. Extracellular and transmembrane domain of TRKC is replaced by PNT domain of ETV6 as the result of t(12;15). C-1 chimeric transcript encodes the complete sequence of the PTK domain, but in C-2 and C-3, the 3'-terminal 462 bp of TRKC is truncated within the PTK domain. Nucleic acid and amino acid sequences surrounding the breakpoint are shown beneath. Vertical arrows indicate the breakpoint. Primers used for RT-PCR are indicated with small arrows. SP, putative signal peptide; TM, transmembrane domain; PTK, protein-tyrosine kinase domain; PNT, pointed domain; ETS, ETS binding domain.

To know whether TRKC was involved in inv(12), we screened the human genome bacterial artificial library (BAC; Research Genetics)with a TRKC cDNA probe and obtained one positive clone, 170I1.FISH analysis was applied to identify the location of the probeon the metaphase of the leukemic cells, which resulted in splitsignals between der(15)(q25) and der(12)(p13) (Figs 1B and 2B).The c-FES probe located telomeric to the TRKC gene hybridizedto normal chromosome 15 and to der(12)(p13). Finally, the karyotypescorrected by FISH analysis were 48,XX,add(6)(q27),+8, der(12)t(12;15)(p13;q25)inv(12)(p13q15),der(15)t(12;15)(p13;q25),+der(15)t(12;15)(p13;q25).

ETV6-TRKC but not TRKC-ETV6 fusion transcript is expressed. Northern blot analysis hybridized with ETV6 full-length cDNA showed previously described transcripts of 6.2, 4.3, and 2.4kb in the t(12;15) leukemic cells and in other leukemic cell lines(Fig 4).¹⁸ On the other hand, a TRKC cDNA probe detected anabnormal 4.3-kb band only in the t(12;15) leukemic cells, comparedwith the 14-kb wild-type message detected in the NBTM cell line.RT-PCR analysis was performed to confirm the fusion transcriptbetween the ETV6 and TRKC gene. We detected an amplified fragmentof expected size using sense primer on ETV6 exon 2 (ETV6-116f)and antisense primer on the PTK domain of TRKC (TRKC-1947r) (Fig5). On the other hand, we could not detect any reciprocal productsof TRKC-ETV6 using the sense primer on the transmembrane domainof TRKC (TRKC-1556f) and the antisense primer on ETV6 exon 5 (ETV6-575r).A normal TRKC message was also undetectable.

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Fig 4. Northern hybridization of t(12;15) leukemic cells. ETV6 full-length cDNA detects 6.2-, 4.3-, and 2.4-kb transcripts (solid arrowhead) in the t(12;15) leukemic cells and Kasumi-1, HL60, and K562 leukemic cell lines (left panel). TRKC probe spanning the breakpoint detects a wild-type 14-kb transcript (solid arrowhead) in the NBTM cell line, whereas a 4.3-kb abnormal band (open arrowhead) is detected in the t(12;15) leukemic cells (right panel). No band is detected in HL60 or K562.

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Fig 5. RT-PCR analysis of ETV6-TRKC fusion products. Total RNA from t(12;15) leukemic cells (lanes 1 through 4) or NBTM cell line (lane 5) was reverse transcribed. PCR amplification was performed using primers ETV6-116f and ETV6-575r (lane 1), ETV6-116f and TRKC-1947r (lane 2), TRKC-1556f and ETV6-575r (lane 3), and TRKC-1556f and TRKC-1947r (lanes 4 and 5), respectively.

Anchored-PCR was performed to confirm whether the reciprocal chimeric ETV6 mRNA exists in the cDNA library. An adaptor primerat the end of cDNA was used as the anchored sense primer and ETV6-541rEprimer was used as the antisense primer. The resulting PCR productswere subcloned into pBluescript phagemid and 30 clones were sequenced,but all the clones encoded only the normal ETV6 sequence. To isolatethe reciprocal chimeric TRKC mRNA, the cDNA library was also amplifiedby the anchored-PCR with TRKC-1602fE primer as the sense primerand an adaptor primer as the antisense primer, but no PCR productwas obtained. Although different types of chimeric mRNA, TRKC-ETV6,and/or TRKC-an unknown gene on 12q15, were suspected to expressin the same leukemic cells, any reciprocal chimeric transcriptsassociating with the 3'-portion of the ETV6 gene or the 5'-portionof the TRKC gene have not been isolated by conventional cDNA screening,RT-PCR, and anchored PCRexperiments.

Expression of ETV6-TRKC fusion protein. To examine whether the chimeric protein was expressed in the leukemic cells, Western blot analysis was performed with an anti-TRKantibody that recognizes the carboxy terminal of the TRK family(TRKA, TRKB, and TRKC). In the NBTM cell line, which expressesTRKA and TRKC, a positive band was detected at 140 to 145 kD ina normal size. On the other hand, an abnormal 52-kD band was detectedin the t(12;15) leukemic cells as the expected size of a C-1 fusiontranscript (Fig 6A). Because the carboxy terminal of TRK proteincontaining the epitope of anti-TRK antibody was deleted in C-2and C-3 protein, the expected 38-kD band of C-2 and C-3 proteincould not be detected. A 140-kD weak band was detected by an anti-TRKantibody in K562 cell line. However, the positive band in K562was derived from TRKA²² but not from TRKC expression, whichwas confirmed by RT-PCR analysis (data not shown). No TRK bandwas detected in other leukemic cell lines such as HL60, Kasumi-1,Kasumi-3, and RS4;11 (data not shown). To determine whether small-sizedfusion protein (C-2 and C-3) are also translated in the leukemiccells, anti-N-TEL antibody was used for Western blot analysis.A 52-kD band, which is the expected size of endogenous ETV6²³and C-1 protein, was detected in all leukemic cells examined.On the other hand, the 38-kD band that reflects the size of theC-2 and C-3 protein was only detected in the leukemic cells witht(12;15) (Fig 6B). Therefore, both types of ETV6-TRKC were expressedin the leukemic cells.

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Fig 6. (A) Abnormal expression of TRKC protein in t(12;15) leukemic cells. Total cell lysates were prepared from NBTM, t(12;15) leukemic cells, HL60 and K562. Wild-type TRK expression is detected in NBTM and weakly in K562. On the other hand, 52-kD abnormal protein is detected only in the t(12;15) leukemic cells. Anti-TRK antibody detects carboxy terminal of the TRK gene family. (B) ETV6/TEL expression in leukemic cells. Western blotting analysis using anti-N-TEL antibody detects a 52-kD band corresponding to the normal ETV6 protein in t(12;15) leukemic cells, HL60, and K562. C-1 ETV6-TRKC protein in t(12;15) leukemic cells is also detected as the 52-kD band. The t(12;15) leukemic cells express a 38-kD protein corresponding to the C-2 and C-3 ETV6-TRKC protein.

  DISCUSSION

We report here an ETV6-associated cryptic translocation t(12;15)(p13;q25) found in an adult patient with AML (M2). The molecularcloning of the ETV6 cDNA showed a novel fusion partner gene, TRKC,which for the first time is reported to be associated with leukemia.TRKC is a receptor tyrosine kinase that is activated by NT-3,a member of the nerve growth factors.²¹ The TRKC gene productencodes three leucine-rich motifs flanked by conserved cysteineresidues and two Ig-like loops in the extracellular domain. Theintracellular domain encodes the well-conserved receptor tyrosinekinase domain, which is a common structure in the TRK subfamilymembers, TRKA, TRKB, and TRKC. TRKC is known to be essential inthe development of the central and peripheral nervous systems.²⁴Expression of TRKC is linked to a favorable outcome in both neuroblastomaand medulloblastoma.²⁵^,²⁶ Activation of TRKA as a result ofrecombination with various genes has been reported in some solidtumors such as colon carcinoma and thyroid carcinoma.²⁷^,²⁸Because abnormality of the TRKC gene in oncogenesis has not beenreported so far, this is the first report that TRKC activationoccurred in a type ofleukemia.

Receptor and nonreceptor tyrosine kinase is known to play an important role in cell growth and differentiation. On the otherhand, activation of these genes by amplification, mutation, orrecombination results in sustained activation of their kinasedomain, which leads to cellular transformation. The BCR-ABL fusiongene, which is observed in t(9;22)-positive chronic myeloid leukemia(CML) or ALL, is one of the well-known models in hematologic malignancies.²⁹Recent studies have shown that some ETV6-associated fusion genes,ETV6-PDGFR $beta$ , ETV6-ABL, and ETV6-JAK2, also have oncogenic propertiesdue to their activated tyrosine kinase activities.⁵^,¹¹^,³⁰^,³¹These fusion transcripts contain the PNT domain of ETV6 that fusedto the catalytic domain of the partner PTK gene. It has been suggestedthat the PNT domain derived from ETV6 contributes to the oncogenicproperties of these chimeric proteins by forming PNT domain-dependenthomo-oligomers that lead to ligand-independent tyrosine kinaseactivation.³⁰^,³¹ TRKC is preferentially expressed in neuraltissues and in some nonneural tissues, but it has not yet beendetected in hematopoietic cells. Taking these findings into consideration,the ETV6-TRKC chimeric transcript, composed of the PNT domainof ETV6 that fused to the PTK domain of TRKC, may possess transformingproperties by aberrantly activated PTK expression in the leukemiccells induced by oligodimerization. In this case, two types ofchimeric transcripts were detected: one included the entire PTKdomain of TRKC (C-1) and the other had the truncated PTK domainof TRKC (C-2 and C-3). These chimeric transcripts may possessdifferent potentials in transforming activities. Further experimentsare needed for addressing the status of these ETV6-TRKC chimericproteins in cells to show the activation mechanism of thiskinase.

In t(12;15), the reciprocal transcript of ETV6-TRKC was not detected and neither was any kind of chimeric mRNA including the3'-portion of ETV6 gene. In t(5;12) and t(9;12), the reciprocaltranscripts of ETV6-PDGFR $beta$ , ETV6-ABL, and ETV6-JAK2 were not detectedeither.²^,⁴^,¹¹ Two kinds of genetic alteration, t(12;15)and inv(12)(p13q15), were found in the leukemic cells. However,the ETV6-TRKC chimeric transcript was only isolated from the breakpoints,suggesting that the ETV6-TRKC transcripts seem to have some rolein leukemogenesis in this type ofleukemia.

The leukemic cells had very aggressive clinical characteristics. The patient's bone marrow was accompanied by severe fibrosisat the time of diagnosis, and the leukemic cells had invaded multipleorgans in a short period.¹⁶ It is not yet clear whether thisdistinct phenotype is due to t(12;15). An accumulation of reportedcases would be needed to discuss this point. Because this translocationis too cryptic to be detected by conventional cytogenetic analysis,FISH or RT-PCR analysis is recommended to study the presence ofthis translocation. The combination of 964c10 YAC and 170I1 BACprobes is an appropriate tool to detect t(12;15) by FISH analysis.One hundred AML patients were screened by the FISH method to seewhether cytogenetically undetected t(12;15) exists, but it hasnot yet been found. t(12;15) seems to be a rather rareevent.

While this report was in preparation, the same ETV6-TRKC fusion gene was reported in cases of congenital fibrosarcoma.³²The reported chimeric transcript encoded exon 1 to exon 5 of theETV6 gene that fused to nt 1741 of the TRKC gene, resulting ina fusion protein functionally resembling the one in our study.There were only two differences between the chimeric transcriptdefined in the leukemic cells and in congenital fibrosarcoma.The first is the existence of ETV6 exon 5 in the chimeric transcriptin the latter case. The second is an additional 14 amino acidinsertion which was observed within the catalytic kinase domainof TRKC (nt 2288) in the case of congenital fibrosarcoma (Fig7). The amino acid insertion occurred just downstream from theTDYYR motif that encompasses the putative autophosphorylationsite of the TRK receptor family.³³^,³⁴ The biological propertiesof this TRKC receptor isoform were previously studied.³³^,³⁵Upon interaction with NT-3, both isoforms became rapidly phosphorylatedon the tyrosine residues and induced DNA synthesis in quiescentcells. However, only TRKC without amino acid insertion had mitogenicactivity in NIH3T3 cells and also induced neuronal differentiationof pheochromocytoma-derived PC12 cells. Moreover, only noninsertiontype TRKC phosphorylated phospholipase C $gamma$ 1 or phosphatidylinositol-3kinase, which is one of the TRKC substrates. These results suggestthat different trophic activities are mediated by TRKC isoforms,which may contribute to the clinical and pathological differencesbetween a very aggressive leukemia and rather benign congenitalfibrosarcoma. There are some examples of genes that affect bothleukemia and solid tumors such as ERG and ALL-1,³⁶^,³⁷ but noidentical fusion transcript has been described in either caseso far. ETV6-TRKC gives a new entity of the fusion gene that mayhave the potential to transform both hematologic and nonhematologiccells.

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Fig 7. Nucleotide and deduced amino acid sequence of the PTK domain of ETV6-TRKC chimeric genes detected in t(12;15)-positive AML (C-1, C-2, and C-3) and congenital fibrosarcoma (CFS). In C-2 and C-3, 3'-terminal 462 bp was truncated within the PTK domain at nucleotide position (nt) 2288 of TRKC, followed by 2 unrelated amino acids and TGA stop codon originating from the intron sequence of TRKC. The number shown above is the amino acid residue in C-1. The nucleotide and deduced amino acid sequence of the 42-bp sequence inserted in the kinase domain in CFS are also indicated. The solid box shows the tyrosine residues (YY) corresponding to the putative major autophosphorylation sites of TRKC.

  ACKNOWLEDGMENT

The authors thank Dr Janet D. Rowley for providing the 964c10 YAC probe, Dr Peter Marynen for providing the LL12NCO1 cosmidprobes, Dr Todd R. Golub for providing TEL cDNA probe, and DrOlivier Bernard for providing anti-N-TEL antibody. We also thankDr Akira Nakagawara for providing NBTM cell line and Dr Eiso Hiyama(Department of General Medicine, Hiroshima University, Schoolof Medicine, Hiroshima, Japan) for providing neuroblastomasamples.

  FOOTNOTES

Submitted May 26, 1998; accepted October 12, 1998.

Supported by a Grant-in-Aid for Scientific Research of Cancer (08266109) from the Ministry of Education, Science, Sports andCulture ofJapan.

The publication costs of this article were defrayed in part by page charge payment. This article must therefore be herebymarked "advertisement" in accordance with 18 U.S.C. section 1734solely to indicate this fact.

Address reprint requests to Nanao Kamada, MD, Department of Cancer Cytogenetics, Research Institute for Radiation Biology and Medicine, Hiroshima University, 1-2-3, Kasumi, Minami-ku, Hiroshima 734-8553, Japan.

  REFERENCES

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Abstract
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© 1999 by The American Society of Hematology. 0006-4971/99/9304-0030$3.00/0

© 1999 by The American Society of Hematology.

0006-4971/99/9304-0030$3.00/0