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Blood, Vol. 91 No. 6 (March 15), 1998:
pp. 1873-1881
By
From the Academic Department of Haematology and Cytogenetics,
Institute of Cancer Research, Haddow Laboratories, Sutton, Surrey, UK;
the Centro de Transplante de Médula Óssea, Instituto
Nacional do Cancer, Rio de Janeiro, Brazil; the Centre for Human
Genetics and Flanders Institute of Biotechnology, University of Leuven,
Leuven, Belgium; and the Department of Cytogenetics, Centre
Régional de Transfusion Sanguine et de Génétique
Humaine, Bois Guillaume, France.
Abnormalities of chromosome 1q21 are common in B-cell malignancies
and have been associated with a poor response to therapy. The nature of
the involved gene(s) on chromosome 1q21 remains unknown. A cell line
(CEMO-1) has recently been established from a patient with
precursor-B-cell acute lymphoblastic leukemia (ALL), which exhibited a t(1;14)(q21;q32). To identify the gene involved in
this translocation, we have cloned both rearranged IGHJ alleles using long-distance inverse polymerase chain reaction (LDI-PCR). Two
IGHJ fragments were amplified from CEMO-1 DNA and sequenced. One allele showed novel sequences upstream of JH5 with no
homology to either IGH or any other sequences on the databases.
Using a single-copy Xho I fragment immediately 5
B-CELL MALIGNANCIES and, in particular,
the B-cell non-Hodgkin's lymphomas (B-NHL) are often associated with
chromosomal translocation in which segments of other chromosomes become
juxtaposed to the IG loci.1 Most of these
involve the IG heavy chain locus (IGH) adjacent to
the telomere of the long arm of chromosome 14 at 14q32.3, but variant
forms may involve the light chain loci at 2p12 (IG The approach of molecular cloning of IGH translocation
breakpoints continues to allow the identification of novel oncogenes and novel pathogenic mechanisms in B-NHL.11-13 To
facilitate the cloning of IGH translocations, we have recently
developed the method of long-distance inverse polymerase chain reaction
(LDI-PCR) for the rapid molecular cloning of such translocation
breakpoints.14
Abnormalities of chromosome 1q21 are a common feature of B-cell
malignancies of all stages of differentiation. No association with a
particular disease subtype has been reported, although abnormalities of
this region have been found in 39% of cases of marginal zone B-cell
lymphoma.15 In B-NHL, 1q21 abnormalities are generally
secondary, occurring in some 10% to 15% of cases, and have been found
by multivariate analysis to be associated with a poor prognosis,
particularly in patients with DLCL.16,17 Abnormalities
include the recurrent translocations t(1;6)(q21;q23-q26), t(1;11)(q21;p15), t(1;12)(q21;q24), t(1;14)(q21;q32), and
t(1;22)(q21;q11)16-18 (I.W., unpublished
observations), together with the duplication dup(1)(q21q32) which, after the MYC translocations, is the
second most common cytogenetic abnormality found in BLs, occurring in greater than 30% of cases.19 However, no oncogene involved
in lymphoid malignancy has yet been identified within this region.
A new pre-B acute lymphoblastic leukemia (ALL) cell line,
CEMO-1
(cIgm+/sIg We report here the molecular cloning using LDI-PCR of the
t(1;14)(q21;q32) in the CEMO-1 cell line, in which IGHJ had
become juxtaposed to novel sequences on 1q21, and the isolation of a new gene (BCL9) of unknown functions. We have also shown that translocation breakpoints in some B-NHL cases with 1q21 breakpoints were located in close proximity to BCL9. In addition, we have found evidence of deregulated overexpression of BCL9 in the
CEMO-1 cell line, suggesting that overexpression of BCL9 may be
of pathogenic significance in a proportion of B-cell malignancies with
breakpoints at 1q21.
Cell lines, cell culture, and cytogenetics.
The CEMO-1 cell line was derived from the peripheral blood of a
previously healthy 30-year-old man with precursor B-cell ALL. He
achieved complete remission after intensive induction therapy, but
sustained a bone marrow relapse 3 months later and died of progressive
disease. Cytogenetic analysis of the original patient material and the
cell line initially showed the presence of the translocation
t(1;14)(q21;q32), but with subsequent growth in vitro the cell line
developed a further t(9;9)(p24;q32). Immunophenotype, cytogenetics and
Southern blot analysis of IGHJ rearrangements have since
remained stable during further culture.20 BL cell lines
were kindly provided by Prof G. Lenoir (IARC, Lyon, France). Details of
these and of other cell lines and their derivation can be obtained on
request. Cell lines were grown in RPMI supplemented with 10% fetal
calf serum under standard conditions.
Southern blot analysis.
DNA blotting was performed as previously described.22
Briefly, high molecular weight DNA was digested with Bgl II,
HindIII, Kpn I, and Xba I (GIBCO-BRL,
Gaithersburg, MD) for 3 to 4 hours at 37°C, electrophoresed in
0.8% agarose and transferred to positively charged nylon membranes
(Hybond N+; Amersham, Amersham, UK) by overnight capillary
transfer. Hybridization to a radiolabeled IGHJ probe (clone
C76R51A) and to BCL9 probes was performed as previously
described.22 Filters were autoradiographed at
LDI-PCR cloning of IGHJ rearrangements.
High molecular weight DNA from CEMO-1 was digested to completion with
HindIII and ligated at low concentration to promote the
formation of monomeric circles. The DNA was then purified using a
Wizard column (Promega, Madison, WI) and 10 ng was amplified in a
nested PCR reaction using primers designed to anneal to the JH
and IGH enhancer regions. The sequences of these primers
were as follows: External J6 (J6E),
5 DNA sequencing.
Automated sequencing was performed using an ABI PRISM automated
sequencer and AmpliTaq polymerase, FS (Perkin Elmer, Foster City, CA).
Sequences were checked against the Genbank and EMBL databases using
BLAST and FASTA programs made available through the Human Genome
Mapping Project Resource Centre (HGMP-RC; Hinxton Hall, Cambridge, UK).
Larger clones were sequenced by primer walking or by subcloning into
pBluescript (Stratagene, La Jolla, CA).
Isolation of PAC and YAC clones and fluorescence in situ
hybridization (FISH).
PAC and YAC clones containing BCL9 sequences were isolated by
radioactive screening using BCL9 cDNA probes from gridded PAC and YAC libraries provided by the HGMP-RC. DNA was extracted from PAC
and YAC clones according to standard techniques.
Northern blot analysis.
A commercial multiple tissue Northern blot with 2 µg poly(A+) RNA
from a variety of tissues (Clontech, Palo Alto, CA) was screened with a
665-bp Xho I fragment single-copy probe (probe X665) derived
from the 1q21 breakpoint region. For cell lines and patient samples,
total RNA was isolated by the guanidium thiocyanate/cesium chloride
method and was electrophoresed on a 1.0% agarose gel containing 2.2 mol/L formaldehyde and transferred to nylon membranes (Hybond N;
Amersham). Hybridization with radiolabeled GAPDH and BCL9
cDNA probes (X665) was performed at 68°C for 90 minutes using Rapid-Hyb buffer (Amersham). The filters were washed with 2× SSC, 0.05% sodium dodecyl sulfate (SDS) at room temperature for 30 minutes
and with 0.1× SSC, 0.1% SDS at 65°C for 30 minutes. Filters were autoradiographed at Isolation of cDNA clones.
cDNA clones were isolated by screening an oligo (dT)-primed normal
human fetal brain cDNA Molecular cloning of a t(1;14) breakpoint in CEMO-1.
Southern blot analysis of HindIII-digested DNA from CEMO-1
using the JH probe showed two rearranged bands of 5.2 and 5.8 kb. These rearrangements were amplified by long-distance inverse PCR, resulting in two products of 3.7 and 4.3 kb
(Fig 1A), which were cloned and sequenced.
Sequence analysis of the 3.7-kb rearrangement showed a productive and
unmutated VH6DIR1DN1JH6 rearrangement (data not shown). In the
other allele, there was loss of homology with IGH sequences
upstream of JH5 (Fig 1B). A restriction map of this 4.3-kb
clone (CH4.3) is shown in Fig 1C. Further sequencing of this clone
showed a region of identity with an EST (accession no.
W23092) cloned from a human retinal cDNA library, but no homology with
any other sequences on the database. A single-copy 665-bp Xho I
fragment (probe X665) containing this region of identity was used to
screen a gridded PAC library, resulting in the isolation of two PAC
clones that were mapped back to chromosome 1q21 on normal metaphases by
FISH (Fig 2A), confirming that this
rearrangement represented the t(1;14) translocation breakpoint. In
addition, the probe X665 gave a rearranged signal on Southern blot that comigrated with the 5.8-kb rearranged JH HindIII
fragment (data not shown).
Isolation of BCL9 cDNA clones.
Because of its identity with an EST, probe X665 was hybridized to
multiple tissue Northern blots containing 2 µg poly(A+) RNA from a
variety of different tissues. Two low-level transcripts were detected
in all tissues, a major transcript of 6.3 kb and a less prominent
4.2-kb species, whereas a third transcript of 1.6 kb was detected only
in spleen, thymus, and, most strongly, in small intestine
(Fig 3).
The translocation t(1;14) in CEMO-1 results in overexpression of
BCL9.
Sequence analysis showed that the t(1;14)(q21;q32) breakpoint in CEMO-1
fell within the 3
Rearrangements of BCL9 in other cases with abnormalities of 1q21.
To assess the extent of involvement of BCL9 in other cases of
B-cell malignancy with abnormalities of 1q21 but in which no RNA was
available, rearrangements of BCL9 were sought in a panel of 39 cases with 1q21 abnormalities. Conventional DNA blot using the 3
In B-cell malignancy, a number of recurrent translocations involving
the IG loci have been characterized. However, a number of
other recurrent cytogenetic abnormalities that only rarely involve the
IG loci have also been identified, some of which are of
prognostic significance. Among these are breakpoints involving 1q21-q23
and 1p32-36, which are associated with a poor prognosis and appear to
exhibit promiscuity in the translocation partners with which they
rearrange.16 In this, both loci are comparable to 3q27, the
location of the BCL6 gene, which has been shown to be
translocated to a large number of loci other than the IG
loci, eg, the t(3;4)(q27;p13) involving the TTF gene at
4p1325 and the t(3;11)(q27;q23) involving the BOB1
gene at 11q23.26
Submitted November 3, 1997;
accepted December 19, 1997.
The authors thank Rifat Hamoudi, Rachel Jackson, Bina Desai, and
Samantha Dibley (Gene Cloning Facility, ICR) for their help with
automated sequencing. We also thank Prof Gilbert Lenoir for kindly
providing the BL lines used in this study and Prof Antonino Carbone
(Centro Regionale di Riferimento Oncologico, INRCCS, Aviano, Italy) for
kindly providing the AS283A cell line.
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Abstract
Introduction
of
JH5, PAC clones were isolated and mapped to chromosome
1q21 on normal metaphases by fluorescence in situ hybridization
(FISH), confirming that this allele represented the
t(1;14)(q21;q32) breakpoint. Sequence analysis of the 1q21 Xho
I fragment showed identity with an expressed sequence tag
(EST), and this probe was therefore used to probe Northern blots. Two transcripts of 6.3 kb and 4.2 kb expressed at low level in
mRNA from all tissues were detected: a third transcript of 1.6 kb was
expressed only in thymus, spleen, and small intestine. Full-length
BCL9 cDNA clones were obtained from a normal human fetal brain
cDNA library supplemented by 5
locus. Other breakpoints were heterogeneous, falling both
centromeric (10 cases) and telomeric (10 cases) of the BCL9
gene. These data suggest that BCL9 may be the target of
translocation in some B-cell malignancies with abnormalities of 1q21
and that deregulated BCL9 expression may be important in their
pathogenesis.
Abstract
) and
22q11 (IG
/CD19+/CD20+/
18. She was admitted in 1995 with gastritis,
leukocytosis, lymphadenopathy, and splenomegaly and died 2 months later
of progressive disease despite multiagent chemotherapy.
Abnormalities of 218 human neoplasms.
Cancer Genet Cytogenet
4:215,
1981
