Molecular Analysis of 11q13 Breakpoints in Multiple Myeloma

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Blood, Vol. 93 No. 4 (February 15), 1999: pp. 1330-1337
Molecular Analysis of 11q13 Breakpoints in Multiple Myeloma

By Domenica Ronchetti, Palma Finelli, Raffaella Richelda, Luca Baldini, Mariano Rocchi, Luigi Viggiano, Antonio Cuneo, Silvia Bogni, Sonia Fabris, Luigia Lombardi, Anna Teresa Maiolo, and Antonino Neri
From the Laboratorio di Ematologia Sperimentale e Genetica Molecolare, Servizio di Ematologia, Università degli Studi di Milano, Ospedale Maggiore IRCCS, Milano; Istituto di Genetica, Università di Bari, Bari; and Dipartimento di Scienze Biomediche e Terapie Avanzate, Università di Ferrara, Ferrara, Italy.

  ABSTRACT

Top
Abstract
Introduction
References

The t(11;14)(q13;q32) chromosomal translocation, which is the hallmark of mantle cell lymphoma (MCL), is found in approximately30% of multiple myeloma (MM) tumors with a 14q32 translocation.Although the overexpression of cyclin D1 has been found to becorrelated with MM cell lines carrying the t(11;14), rearrangementsof the BCL-1/cyclin D1 regions frequently involved in MCL rarelyoccur in MM cell lines or primary tumors. To test whether specific11q13 breakpoint clusters may occur in MM, we investigated a representativepanel of primary tumors by means of Southern blot analysis usingprobes derived from MM-associated 11q13 breakpoints. To this end,we first cloned the breakpoints and respective germ-line regionsfrom a primary tumor and the U266 cell line, as well as the germ-lineregion from the KMS-12 cell line. DNA from 50 primary tumors wastested using a large panel of probes, but a rearrangement wasdetected in only one case using the KMS-12 breakpoint probe. Ourresults confirm previous findings that the 11q13 breakpoints inMM are scattered throughout the 11q13 region encompassing thecyclin D1 gene, thus suggesting the absence of 11q13 breakpointclusters inMM.
© 1999 by The American Society of Hematology.

  INTRODUCTION

Top
Abstract
Introduction
References

CHROMOSOMAL translocations affecting the immunoglobulin heavy chain (IGH) locus on 14q32 represent the mechanism ofactivation of a number of proto-oncogenes in B-cell lymphoid neoplasms.¹The t(11;14)(q13;q32) chromosomal translocation is associatedwith approximately 70% to 90% of mantle cell lymphomas (MCL)^2-5and leads to the overexpression of the cyclin D1 gene.^6-9 Thebreakpoints on chromosome 11q13 were initially found clusteredin a 1-kb region, named the major translocation cluster (MTC),of the BCL-1 locus.² Further investigations have shown thatbreakpoints may occur telomeric of the MTC in a region of about120 kb between the MTC and the cyclin D1 loci.³ Molecular analyses,including fluorescence in situ hybridization (FISH), have alsodemonstrated that breakpoints may occur either centromeric ortelomeric of this 120 kb region in some cases.⁴^,⁵^,⁹

Multiple myeloma (MM) is a malignant proliferation of bone marrow plasma cells that is characterized by a wide spectrum ofclinical entities and whose molecular pathogenesis is still largelyunknown.^10-11 Cytogenetic analyses in MM are limited and difficultmainly because of the low proliferation rate of malignant plasmacells. However, in about 20% to 40% of tumors with an abnormalkaryotype, a 14q⁺ marker has been reported.¹²^,¹³ This marker is generally theconsequence of translocation events involving the IGH locus onchromosome 14q32. Interestingly, in almost 30% of cases with cytogeneticallydetectable 14q⁺, the marker is the result of a t(11;14)(q13;q32) chromosomaltranslocation. However, rearrangements of the BCL-1/cyclin D1regions frequently involved in MCL rarely occur in MM.⁹^,^14-16Molecular characterization of breakpoints in a limited numberof MM-derived cell lines carrying the t(11;14)(q13;q32) chromosomaltranslocation suggested that they are scattered over a relativelylarge area encompassing the BCL-1/cyclin D1 region.⁹^,¹⁶ However,overexpression of cyclin D1 is generally associated with the t(11;14)in MM cell lines, thus suggesting that it represents the targetgene of the translocation.⁷^,⁹^,¹⁶ Therefore, the currentlyavailable probes specific for the 11q13 breakpoints may not beuseful for detecting BCL-1/cyclin D1 rearrangements inMM.

In an attempt to investigate this point further, we cloned the genomic regions from the 11q13 breakpoints of three differentMM cases (two cell lines and a primary tumor). The breakpointswere scattered along the 11q13 region at various distances fromthe cyclin D1 locus, as observed by FISH analysis. Specific 11q13probes from these regions were used in Southern blot analysesto search for genomic rearrangements in a representative panelof primary MM tumors that had been previously found to be negativefor BCL-1/cyclin D1 rearrangements. With these new probes, wewere able to detect rearrangements in only one of the 50 MM tumorsinvestigated. Our results confirm previous findings that 11q13breakpoint in MM are scattered over the 11q13 region encompassingthe cyclin D1 gene and suggest the absence of 11q13 breakpointclusters inMM.

  MATERIALS AND METHODS

Pathological samples. Bone marrow or peripheral blood samples from 50 MM patients investigated by Southern blot analysis were collected during thecourse of standard diagnostic procedures. The diagnosis and clinicalstaging of MM was made according to the criteria described byDurie and Salmon.¹⁷ These samples came from a larger seriesof 88 previously investigated primary MM tumors.¹⁸ Forty patientswere at first diagnosis: six in stage I (indolent phase), 22 instage II, and 12 in stage III; five patients were evaluated atclinical relapse and five were affected by plasma cell leukemia(four at diagnosis and one at relapse). Twenty-one of the patientswere male and 29 female; their median age was 61 years (range,42 to 80). Monoclonal component was as follows: IgG (35 patients),IgA (11), $kappa$ / $lambda$ chain 30/16; $kappa$ chain (3) $lambda$ chain (1). No conventionalcytogenetic analyses (G-banding) of these samples wereavailable.

The previously reported tumor LB411¹⁸ was derived from a 69-year old male patient affected by IgGk-type plasma cell leukemiawith 2 months survival; no karyotype was available in this case.Case AC97 was a 74-year-old female with a $kappa$ -type MM in clinicalstage III that had the following karyotype: 46,XX, del(1)(p13p22),inv(9)(p12;q13), t(11;14)(q13;q32), del(13)(q22q31). The patientshowed a partial clinical response to conventional chemotherapyand is still alive 2 years afterdiagnosis.

The MM-derived cell lines U266 and KMS-12 have been previously reported; a cytogenetically detectable t(11;14)(q13;q32) chromosomaltranslocation has been found in the KMS-12, but not the U266 cellline.¹⁹^,²⁰ No evidence of any rearrangement of the BCL-1 locusor cyclin D1 gene has been observed in either cell line, whereascyclin D1 overexpression has been detected in both⁷^,¹⁶ (andpresent study). The U266 cell line was obtained from the AmericanType Culture Collection (Rockville, MD); the KMS-12 cell linewas kindly provided by Dr T. Otsuki (Okayama,Japan).

DNA preparation and Southern blot analysis. Mononuclear cell suspensions with more than 95% viability were prepared from the pathological samples by means of Ficoll-Hypaquegradient centrifugation; the percentage of malignant plasma cellsidentified by immunocytomorphologic analyses was between 22% and98%. DNA from pathological samples and cell lines was purifiedby proteinase K digestion, phenol-chloroform extraction, and ethanolprecipitation.²¹ A total of 10 µg of genomic DNA was digestedwith BamHI, EcoRI, or HindIII restriction enzymes, electrophorizedin a 0.7% agarose gel, and then denaturated, neutralized, andtransferred to nylon filters (Amersham International, Amersham,UK). The filters were hybridized to ³²P-labeled probes according to the manufacturer's specifications,washed in 0.5 × SSC (NaCl/Na citrate)/1% sodium dodecyl sulfate(SDS) for 1 hour at 60°C and then autoradiographed using an intensifyingscreen at $-$ 80°C.²¹ IGH gene rearrangement was analyzed usingpreviously described probes^22-24; the probes used for the rearrangementanalysis of the BCL-1/cyclin D1 locus were MTC, p94, and cyclinD1 cDNA.²^,³^,⁶

Molecular cloning. The identification of a t(11;14)(q13;q32) chromosomal translocation in one primary case of MM (LB411) and the U266 cell linewas made possible following a Southern blot approach recentlyreported by us,¹⁸ which allows the identification of putativeswitch-translocated IGH alleles on the basis of the absence ofany linkage between different IGH regions. A quite similar approachhas been previously reported by others.²⁵ We reasoned that,as a result of immunoglobulin gene recombination during maturationof B cells, the rearranged joining-switch-constant IGH regionsare generally contained on a novel BamHI restriction fragment,and that a translocation event involving the switch region shouldtherefore generate a rearranged BamHI fragment containing the3' constant region, but not the 5' joining sequences of the IGHgene. In our Southern blot assay, the DNA was digested with BamHIrestriction enzyme, and the filters subsequently hybridized withthe JH, Cµ, C $alpha$ 1, and C $gamma$ 1 probes. The identification of rearrangedIGH alleles as potential candidates for switch-mediated chromosomaltranslocations was based on the absence of comigration betweenthe DNA fragments containing constant IGH regions and those positivefor the JH probe. Recombinant phage clones containing translocatedC $alpha$ -rearranged IGH alleles from case LB411 and the U266 cell linewere obtained by complete digestion of genomic DNA with BamHI,the subsequent ligation of gel-purified fractions into $lambda$ EMBL3phage vectors (Stratagene, La Jolla, CA) and screening with theC $alpha$ 1 probe. The germ-line regions of chromosome 11 were isolatedby screening a genomic library of human placenta DNA (Clontech,San Diego, CA) using probes derived from recombinant clones. Thenormal 11q13 region encompassing the breakpoint in KMS-12 wascloned by screening a phage genomic library with a 193-bp fragmentspecific for the KMS-12 breakpoint region, which was obtainedby polymerase chain reaction (PCR) amplification of genomic DNAusing a pair of previously reported primers.¹⁶ The library screeningand plaque isolation were performed according to established procedures.²¹The inserts were analyzed using restriction enzyme mapping andthen subcloned into plasmid vector pGEM3 (Promega, Madison,WI).

DNA sequencing. DNA sequence analysis was performed on restriction fragments cloned into pGEM3 plasmid (Promega) by "dideoxy" chain-terminationanalysis using the Sequenase sequencing kit (USB, Cleveland,OH).

cDNA amplification. The synthesis of the first strand cDNA was performed as previously described.¹⁸ PCR amplifications were made by diluting5 µL of first-strand cDNA from each individual case into a 50-µLPCR mixture. A 196-bp fragment encompassing exons 3 and 4 of cyclinD1 gene⁶ was amplified using the following primers: sense 5'-AACAGATCATCCGCAAACAC-3';antisense 5'-TCACACTTGATCACTCTGGA-3'. Thirty cycles of amplificationwere performed at 94°C for 30 seconds, 60°C for 30 seconds, and72°C for 30seconds.

FISH. The chromosome preparations were hybridized in situ with probes labeled with biotin or directly with the fluorochrome, Cy3(Amersham, Little Chalfont, UK) by nick translation, as described²¹with minor modifications.²⁶^,²⁷ Briefly, 200 ng of labeled probewere used for each experiment, and hybridization was performedat 37°C in 2 × SSC, 50% (vol/vol) formamide, 10% (wt/vol) dextransulphate, 5 µg Cot1 DNA (Boehringer, Mannheim, Germany), and 3µg of sonicated salmon sperm DNA in a volume of 10 µL. Posthybridizationwashing was at 60°C in 0.1 × SSC (three times). Biotin-labeledDNA was detected using fluorescein isothiocyanate (FITC)-conjugatedavidin (Vector Laboratories, Burlingame, CA). The chromosomeswere identified by simultaneous 4',6'-diaminido-2-phenylindoledihydrochloride (DAPI) staining, which produces a Q-banding pattern.Chromosome 11 and 14 painting probes were obtained by Alu-PCRamplification of the somatic cell hybrids retaining only the humanchromosome 11 or 14.²⁸ Digital images were obtained using aLeica DMR epifluorescence microscope equipped with a CCD camera(Cohu, Inc, San Diego, CA). FITC-avidin, Cy3, and DAPI fluorescencesignals were detected using specific filters and recorded separatelyas gray scale images. Pseudocoloring and image merging were performedusing Adobe Photoshop software (Adobe Systems, Mountain View,CA).

Probes for FISH analysis. The probes used are described in Fig 1. The cosmid clones representative of the cyclin D1 and FGF3 loci were isolated by screeninga cosmid library of human placenta (Clontech) with probes specificfor cyclin D1⁶ or FGF3/int-2 cDNA.²⁹ The FGF4/hst-1 locus was investigatedusing an 8-kb genomic fragment containing the 5' of the gene.³⁰The cosmid clones I4, R4B, and pHS-11 encompassing the MTC regionhave been previously described.⁹ All of the YACs were obtainedfrom the human CEPH2 library (YAC Screening Center, DIBIT, Milan,Italy): YAC clones 961-H-2 (800 kb) and 744-F-12 (330 Kb) havebeen previously reported³¹ and are both negative for the MTCregion; YAC clone 877-D-8 (1080 kb) was identified by the presenceof the D11S911 marker, telomeric of the GARP locus on 11q14.⁹^,³²The IGH locus was analyzed using a phage clone containing the18-kb C $alpha$ 1 BamHI germ-line fragment.²³

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Fig 1. Schematic representation of the chromosome 11q13-11q14.1 probes used for the molecular and FISH analyses. See Materials and Methods for further details.

  RESULTS

Cloning of a t(11;14)(q13;q32) in a MM primary tumor. We have recently reported the identification of IGH rearranged alleles as potential candidates for switch-mediated chromosomaltranslocations in 21 of 88 cases of primary MM tumors investigated.¹⁸To confirm the presence of chromosomal breakpoints in these alleles,we cloned the rearranged fragments from three cases (two C $alpha$ andone Cµ rearrangement). In two of these tumors, molecular cloningand FISH analyses showed the presence of a novel t(4;14)(p16.3;q32)chromosomal translocation.¹⁸ In the third MM tumor (case LB411),a t(11;14)(q13;q32) chromosomal translocation was identified bycloning a 10-kb BamHI C $alpha$ 1 rearranged fragment (Fig 2) that wasapparently negative for JH sequences.¹⁸ This fragment was isolatedas described in Materials and Methods and used as a probe in theFISH analysis of metaphase spreads from mitogen-stimulated normalperipheral blood lymphocytes. This clone hybridized to both chromosome14q32 and chromosome 11q13, thus indicating that the rearrangementwas a result of a t(11;14)(q13;q32) chromosomal translocation(data not shown). About 25 kb of the normal genomic region surroundingthe breakpoint on chromosome 11q13 were cloned by isolating twooverlapping phages from a normal genomic library (Fig 2). Noneof this genomic region hybridized with probes specific for theBCL-1 locus (MTC, p94, and full-length cyclin D1 cDNA), thus confirmingthe absence of rearrangements in these regions observed in Southernblot analysis of LB411 DNA (data not shown). Subsequently, thisregion was hybridized with a set of 11q13 genomic clones (seeFig 1); cosmids R4B and pHS-11 were both positive, thus indicatingthat the breakpoint in case LB411 occurred approximately 40 to45 kb telomeric of the MTC region and consequently 65 to 70 kbcentromeric of the cyclin D1 gene. Interestingly, reverse transcriptase(RT)-PCR analysis showed that this case was overexpressing cyclinD1 (data not shown).

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Fig 2. Molecular cloning of the chromosomal breakpoint from case LB411. (A) Schematic representation of the breakpoint and the respective 11q13 germ-line region. From the top: a diagram of the BCL-1/cyclin D1 locus where the cosmid clones I4, R4b, pHS11 are located is shown; the 11q13 germ-line region and the probes used for the Southern and Northern blot analyses are shown as solid lines. The vertical arrow indicates the breakpoint position. In the t(11;14) breakpoint clone, chromosome 14 is indicated by open boxes with black or stippled boxes representing different IGH regions and chromosome 11 is shown as a solid line. Restriction enzyme symbols: B, BamHI; R, EcoRI; H, HindIII; X, XhoI. (B) The nucleotide sequence of the breakpoint region and its alignment with 11q13 and 14q32 germ-line sequences are shown.

Cloning and mapping of the 11q13 breakpoint in MM cell line U266. We investigated cyclin D1 expression in a panel of MM-derived cell lines (U266, KMM1, JJN3, OPM2, Karpas, IM9, Sultan, LP-1)for which karyotypic analyses have been reported to be negativefor the t(11;14)(q13;q32) chromosomal translocation. Interestingly,Northern blot analysis demonstrated a high level of cyclin D1expression in U266 cell line (Fig 3A). On the basis of this evidence,we looked for the presence of an illegitimate IGH recombinationin U266 DNA by Southern blot, as for case LB411. As shown in Fig3B, hybridization of BamHI-digested DNA with the C $alpha$ 1 probe detecteda rearranged fragment that did not comigrate with the rearrangedJH allele. A phage library was constructed using BamHI-digestedDNA from the U266 cell line and screened with the C $alpha$ 1 probe. Therearranged C $alpha$ 1 fragment was isolated and tested on normal metaphasesby FISH analysis, which showed hybridization with chromosomes14q32 and 11q13 (data not shown) that was consistent with thepresence of a t(11;14)(q13;q32) chromosomal translocation. Wenext cloned about 20 kb of the normal genomic region surroundingthe breakpoint by isolating a recombinant phage from a normalgenomic library (Fig 3C). This genomic region did not hybridizewith MTC, p94, or full-length cyclin D1 cDNA and with any of theavailable 11q13 clones (see Fig 1).

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Fig 3. Molecular analysis of the U266 MM cell line. (A) Northern blot analysis of human MM cell lines showing cyclin D1 overexpression in U266. The length of the cyclin D1 transcripts is shown in kb. $beta$ -actin hybridization is shown for loading quantification. (B) Southern blot analysis of the IGH locus in the U266 cell line. The DNA was digested with BamHI restriction enzyme, and the nylon filter was subsequently hybridized with the probes specified below. The germ-line bands are indicated by dashes. The arrow indicates the cloned "illegitimate" IGH rearranged fragment. (C) Molecular cloning of the chromosomal breakpoint in the U266 cell line. The breakpoint and the respective 11q13 germ-line region are shown; the probes used for Southern and Northern blot analyses are shown in the diagram. The vertical arrow indicates the breakpoint position. Chromosome 14 is represented by open boxes with black or stippled boxes showing different IGH regions and chromosome 11 is represented as a solid line. Restriction enzyme symbols: B, BamHI; R, EcoRI; H, HindIII; X, XhoI. (D) The nucleotide sequence of the breakpoint region and its alignment with 14q32 and 11q13 germ-line sequences are shown.

To define the location of the U266 11q13 breakpoint more precisely, we performed FISH analyses on metaphases spreads. As shownin Fig 4A, the chromosome 11 painting probe hybridized with twochromosomes on U266 metaphases: an apparently normal chromosome11 and a structurally altered chromosome consisting of the 11pter $right-arrow$ 11q13-14region and extra material of unknown origin. Hybridizations withprobes specific for the MTC region, and the cyclin D1, FGF4, andFGF3 loci, indicated that all of these regions are contained inthe putative 11q13 region of this abnormal chromosome (data notshown). Hybridization with the chromosome 14 painting probe clearlydetected two different chromosomes: an apparently normal chromosome14 and an abnormal chromosome with a large amount of chromosome14 material on its long arm. (Fig 4B). Thus, no detectable exchangeof material between chromosomes 11 and 14 was observed with paintingprobes hybridization: a finding consistent with the absence ofa cytogenetically detectable t(11;14)(q13;q32) in U266 cell line.Interestingly, the C $alpha$ 1 clone was clearly detected at 11q13-14on the abnormal chromosome 11 (colocalized with each of the 11q13probes tested above; Fig 4C and data not shown), as well as inthe telomeric region of both chromosomes recognized by the 14painting probe (Fig 4C). These findings indicated the presenceof a t(11;14) and suggested that the breakpoint on 11q13 may belocated telomeric of the FGF3 locus. Interestingly, the YAC clone877-D-8 specific for a region telomeric of the GARP locus on 11q14hybridized to the abnormal chromosome 11 in U266 metaphases, thussuggesting that this locus is still retained. Triple-hybridizationexperiments using MTC (green), C $alpha$ 1 (red), and 877-D-8 (green)probes showed that the C $alpha$ region is apparently located betweenthe MTC and GARP loci (Fig 4C). These findings indicate that thet(11;14) translocation in U266 is the result of a complex chromosomerearrangement, as is also suggested by the presence of extra materialon the abnormal chromosome 11. The FISH experiments performedin an attempt to elucidate the origin of the extra material onthis chromosome gave very complex results; however, chromosomes3 and 4 are apparently involved (data not shown).

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Fig 4. FISH analysis of the U266 MM cell line. (A) Partial U266 metaphase hybridized with the chromosome 11 painting probe. (B) Partial U266 metaphase hybridized with the chromosome 14 painting probe. DAPI counterstaining is shown for each chromosome. (C) Partial U266 metaphase cohybridized with cosmid I4 (green), YAC 877-D-8 (green), and C $alpha$ 1 (red) probes. For details concerning these probes, see text and Fig 1.

Mapping of 11q13 breakpoints in MM tumors with a cytogenetically detectable t(11;14)(q13;q32) chromosomal translocation. We used FISH analysis to investigate the approximate location of the 11q13 breakpoints in the cell line KMS-12 and a primaryMM tumor (AC97), both carrying a t(11;14)(q13;q32) chromosomaltranslocation.

While this work was in progress, Chesi et al¹⁶ reported the cloning of a t(11;14) breakpoint in the KMS-12; more recently,Vaandrager et al³³ have reported that this breakpoint is locatedapproximately 215 kb centromeric of the MTC region and is juxtaposedto the C $gamma$ 2 of the IGH locus. Therefore, only part of our resultswill be presented. In particular, double-color FISH on KMS-12metaphase spreads with the painting probes specific for chromosomes11 and 14 showed the presence of five putative 14 (der) chromosomescontaining material from chromosome 11 (Fig 5A1). FISH analysesfurther demonstrated that the MTC, cyclin D1, FGF4, and FGF3 lociwere all contained in these chromosomes and apparently juxtaposedto sequences recognized by the C $alpha$ 1 probe (Fig 5A2 and data notshown). The YAC clones 961-H-2 and 744-F-12 located centromericof the MTC region (see Fig 1) did not hybridize with the 14 (der)chromosomes (Fig 5A3 and data not shown), but with two small andstructurally-altered chromosomes recognized by the painting andcentromeric-specific probes of chromosome 11 (Fig 5A1, 3, anddata not shown). These results suggest that the breakpoint iscentromeric of the MTC region and are consistent with previouslyreported data.³³

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Fig 5. FISH analysis of the 11q13 breakpoints in MM tumors with a cytogenetically detectable t(11;14)(q13;q32) chromosome translocation. (A) FISH analysis of the KMS12 cell line: (1) partial metaphase cohybridized with chromosome 11 (green) and chromosome 14 (red) painting probes; (2) partial metaphase cohybridized with cosmid I4 (MTC-green) and C $alpha$ 1 (red) probes; (3) partial metaphase cohybridized with YAC 961-H-2 (red) and C $alpha$ 1 (green) probes. DAPI counterstaining is shown for each chromosome. (B) Double-color interphase FISH analysis of MM tumor AC97. Left: colocalized signals in cohybridization experiments with YAC 744-F-12 (green) and pHS11 (red) probes; right: dissociated signals in cohybridization experiments with pHS11 (red) and cyclin D1 (green) probes. See scheme in Fig 1 for the probes used.

Case AC97 carried a t(11;14)(q13;q32) chromosomal translocation (see Materials and Methods; data not shown) without any evidenceof the involvement of the BCL-1/cyclin D1 regions at Southernblot analysis (data not shown). No data concerning cyclin D1 expressionwere available in this case. Two-color FISH analysis in interphasenuclei with probes of the 11q13 region showed that the breakpointin this case is apparently located between MTC and the cyclinD1 locus. In particular, colocalization of signals (red and green)were detected on interphase nuclei when YAC 744-F-12 was usedtogether with the pHS11 clone (Fig 5B) and when the cyclin D1cosmid was cohybridized with the FGF3-specific clone (data notshown), but dissociation of signals was observed when the pHS11and cyclin D1 cosmids were used (Fig 5B).

Lack of clusters of 11q13 breakpoints in MM. Because the t(11;14)(q13;q32) translocation is recurrently found in MM, we investigated by Southern blot whether any of thecloned 11q13 breakpoints were involved in the translocation inother MM cases using the probes described in Fig 6, which arespecific for case LB411 and cell lines U266 and KMS-12. We testedDNA from 50 MM primary tumors for which karyotype data were notavailable. Furthermore, all of these cases have been found tobe negative for rearrangements of the MTC and p94 regions andcyclin D1 locus (data not shown). Southern blot analysis was performedon BamHI DNA digests and, when possible, on EcoRI and HindIIIdigests. Rearrangements were detected in only one tumor (patientLB104) and involved the 11q13 region where the breakpoint of theKMS-12 cell line is located (Fig 6). Case LB104 was a 72-year-oldfemale patient affected by an IgA $lambda$ -type MM in clinical stage IIAat diagnosis and with 32 months survival. Cyclin D1 expressionwas evaluated by RT-PCR in only 11 of the 50 MM patients (includingcase LB104). Specific amplified fragments were detected in caseLB104 and in an IgG $lambda$ -type MM tumor (case LB413) from a 75-year-oldfemale patient in clinical stage IIIB at diagnosis with 13 monthssurvival (data not shown).

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Fig 6. Southern blot analysis of MM tumors using 11q13 probes. (A) DNA was digested with HindIII restriction enzyme and hybridized with the 193 bp probe (see Materials and Methods) located in proximity of the KMS-12 breakpoint¹⁶; a rearrangement was observed in one tumor (case LB104; see text). (B) DNA was digested with BamHI restriction enzyme and hybridized with the A/H 0.6 kb probe located in proximity of the LB411 breakpoint. (C) DNA was digested with HindIII restriction enzyme and hybridized with the B/R 0.4 kb probe located in proximity of U266 breakpoint. The rearrangement patterns of KMS12, LB411, and U266 with the specified 11q13 probes are respectively shown in (A, B, and C). Germ-line fragments are indicated by dashes. The diagrams represent the 11q13 germ-line regions; probes used in the Southern blot analyses are shown. Restriction enzyme symbols: H, HindIII; B, BamHI; R, EcoRI; A, AvaI.

  DISCUSSION

Conventional cytogenetic analyses of MM are generally a difficult task because of the low proliferation rate of malignantplasma cells. Abnormal karyotypes have been reported only in about40% of MM and at a higher frequency in plasma cell leukemia; interestingly,in about 20% to 40% of MM patients with an abnormal karyotypea 14q⁺ marker is observed.¹²^,¹³ In about 30% of the cases, the 14q⁺ marker originates through a t(11;14)(q13;q32) chromosomal translocation,which is mainly associated with MCL and involves the cyclin D1gene on 11q13.¹² However, rearrangements of the BCL-1/cyclinD1 regions involved in MCL have been rarely demonstrated in casesof MM carrying such a translocation (mainly cell lines) or inunselected tumors.⁹^,^14-16 The overexpression of cyclin D1 hasbeen observed in the majority of MM-derived cell lines carryingthe t(11;14), thus suggesting that this translocation may leadto the disregulation of this gene in MM, as it does in MCL.⁷^,⁹^,¹⁶The main aim of the present study was to investigate whether specificregions on 11q13 are associated with 11q13 breakpoints in MM.To this end, we cloned and mapped different 11q13 breakpoints,isolated the corresponding germ-line regions, and evaluated inSouthern blot a representative panel of MM primary tumors forgenomicrearrangements.

In case LB411, the breakpoint was located between MTC and cyclin D1, approximately 40 kb telomeric of the MTC. In case AC97carrying a t(11;14), FISH analysis allowed us to map the breakpointin this region, in which the breakpoints from the MM cell linesXG1 and SK-MM2 have also been found to be located.⁹^,¹⁶ Inthe U266 cell line, the breakpoint is telomeric of the cyclinD1 locus between the FGF3 and GARP loci; however this rearrangementis complex because the C $alpha$ 1 region is located to the abnormal chromosome11, and apparently the GARP locus is still retained on this chromosome.As far as we know, this is the second MM tumor in which the 11q13breakpoint has been mapped telomeric of cyclin D1. Raynaud etal⁹ reported a similar finding in the XG2 cell line; however,the cyclin D1 gene was not found to be expressed in this cellline. Given the large distance between FGF3 and GARP, it can besuggested that the breakpoint in U266 may be closer to the FGF3gene, at a distance that can affect cyclin D1 expression. In theKMS-12 cell line, the breakpoint is centromeric of the MTC. Duringthe course of this study, Vaandrager et al³³ reported that thebreakpoint in this cell line is located 215 kb centromeric ofthe MTC region; Southern blot analysis showed that the breakpointin our case LB104 appears to be located in the same region. Abreakpoint centromeric of the MTC locus has been previously reportedin the XG5 MM cell line.⁹ Taken together, these data confirmthe notion that 11q13 breakpoints in MM are scattered along the11q13 (see scheme in Fig 7) and suggest that they may occur eithercentromeric of the MTC, between the MTC and cyclin D1 loci, ortelomeric of the cyclin D1. Interestingly, we found by RT-PCRthat the presence of 11q13 breakpoints in tumors LB411 and LB104correlates with cyclin D1 overexpression (data not shown).

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Fig 7. Schematic representation of the MM breakpoints location in the 11q13 region. For details, see Raynaud et al⁹ (XG1,XG2,XG5 cell lines), Meeus et al¹⁵ (two MM cases), Chesi et al¹⁶ (SK-MM2 cell line), and Vaandrager et al³³ (KMS-12 cell line). The arrows indicate cases for which the breakpoint has been cloned; the dashes indicate cases for which the breakpoint has been approximately mapped by FISH or Southern blot analyses.

The availability of 11q13 probes specific for breakpoints in MM would make it possible to investigate by Southern blot analysiswhether distinct breakpoint clusters may occur in MM. As far aswe know, this is the first study regarding the screening of MMtumors using such an approach; however, our analysis with probesfrom three distinct 11q13 regions representative of MM breakpointsdetected a rearrangement in only one case, further confirmingthe notion that 11q13 rearrangements associated with MM are scatteredover a large region encompassing the cyclin D1 gene. These findingssuggest that other technical approaches, such as FISH on interphasenuclei,⁴ are needed to assess the frequency and involvementof 11q13 breakpoints inMM.

  AKNOWLEDGMENT

We are grateful to Dr S. Raynaud and P. Delli Bovi for providing us with cosmid clones I4, R4B, pHS-11, and FGF4 clone, respectively,and to Dr T. Otsuki for providing us with the KMS-12 cell line.We thank G. Ciceri for her expert technicalassistance.

  FOOTNOTES

Submitted June 17, 1998; accepted October 6, 1998.

Supported by grants from the Associazione Italiana Ricerca sul Cancro (AIRC) (to A.N. and M.R.) and the Ministero della Sanitàto Ospedale Maggiore IRCCS (Ricerca Corrente1994).

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 Antonino Neri, MD, Servizio Ematologia Istituto di Scienze Mediche, Università di Milano, Ospedale Maggiore di Milano, IRCCS Via Francesco Sforza 35, 20122 Milano, Italy; e-mail: filobus{at}imiucca.csi.unimi.it.

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Abstract
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© 1999 by The American Society of Hematology. 0006-4971/99/9304-0004$3.00/0

© 1999 by The American Society of Hematology.

0006-4971/99/9304-0004$3.00/0