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Blood, Vol. 91 No. 12 (June 15), 1998:
pp. 4677-4685
By
From the Hematopathology Section, Laboratory of Pathology, National
Cancer Institute, National Institutes of Health, Bethesda, MD; and the
Department of Pathology, British Columbia Cancer Agency, Vancouver,
British Columbia, Canada.
Low-grade follicle center lymphoma (LGFCL) is characterized
genetically by the t(14;18) translocation and an indolent clinical course. Histologic progression from LGFCL to an aggressive diffuse large B-cell lymphoma (DLCL) occurs in 60% to 80% of cases, and this
transformation is associated with the accumulation of secondary genetic
alterations. Using 10 polymorphic microsatellite markers spanning the
chromosome 9p21 region harboring the p15
(p15INK4B/MTS-2/CDKN2B) and p16
(p16INK4A/MTS-1/CDKN2) tumor-suppressor gene loci, we
analyzed 11 matched pairs of LGFCL and their corresponding progressed
DLCL biopsies for loss of heterozygosity and homozygous deletions at
9p21. A comparative multiplex polymerase chain reaction assay was also used for the detection of homozygous deletions. Deletions were identified in 8 of the 11 cases studied (73%): 6 homozygous (54%) and
2 hemizygous (18%). The deletions were identified exclusively in the
progressed DLCL biopsies. Immunohistochemical studies showed an
excellent correlation with the results from the genetic analyses. Of
the 9 matched pairs of LGFCL and progressed DLCL with interpretable immunohistochemical staining, 9 of 9 (100%) of the LGFCL showed diffuse reactivity for p16. Four of the 9 (44%) immunohistochemically evaluable cases of progressed DLCL showed loss of or, in 1 case, markedly diminished p16 expression. All 4 of these cases
correspondingly showed homozygous deletions at 9p21. Five of the 9 progressed DLCL cases showed p16 expression and demonstrated retention
of one or both 9p21 alleles by genetic analysis. This is the first longitudinal series examining sequential biopsy specimens of low-grade and progressed FCL for genetic loss at 9p21 encompassing the p16 and
p15 loci. The high frequency and exclusive occurrence of deletions involving p16 in the progressed DLCLs suggests that genetic loss at
9p21 targeting p16 and/or p15 is an important secondary genetic event in the histologic progression of FCL.
FOLLICLE CENTER lymphoma (FCL) accounts
for approximately 40% of adult non-Hodgkin's lymphomas in the United
States.1 Although most patients present with advanced stage
disease at diagnosis, the clinical course is generally indolent.
Histologic progression from a low-grade to a diffuse aggressive
lymphoma occurs in approximately 60% to 80% of cases.2,3
This transformation is usually associated with a rapidly progressive
clinical course and a short survival.4-6
The t(14;18)(q32;q21) chromosomal translocation that juxtaposes the
bcl-2 protooncogene (band 18q21) to the Ig heavy chain joining region
(band 14q32)7,8 is detectable in up to 90% of cases of
FCL.9 This molecular event results in the deregulation of
bcl-2 gene expression, and elevated levels of bcl-2 mRNA and protein.10,11 Overexpression of bcl-2 protein is thought to inhibit apoptosis and results in the accumulation of follicle center
cells with increased survival.10,11 The accumulation of
additional secondary genetic alterations in centrocytes bearing the
t(14;18) translocation,12 such as p5313 and myc
mutations,14 is associated with the evolution and
progression of FCL.
The genes for the cyclin-dependent kinase (CDK) inhibitors, p15
(p15INK4B/MTS-2/CDKN2B) and p16
(p16INK4A/MTS-1/CDKN2), have recently been mapped to
chromosome 9p21.15 These genes encode small nuclear
proteins that have been shown to block cell cycle progression at the
G1/S transition by their ability to interfere with the catalytic
activity of cyclin D/CDK4 complexes.16 Active cyclin D/CDK4
complexes are necessary for phosphorylation of the Rb protein and for
the subsequent release of critical transcription factors, such as E2F,
that are required for progression into S phase. p16 is therefore an
attractive candidate for a tumor-suppressor gene, because loss of its
function could potentially lead to uncontrolled cell
growth.15,16 The p15 gene, located approximately 25 kb
centromeric to p16, exhibits structural homology to p16 and also
demonstrates cyclin D/CDK 4 kinase inhibitor activity. The structural
and functional similarities of p15 to p16 suggest that p15 is also a
candidate tumor-suppressor gene.
That p16 and potentially p15 are in fact tumor-suppressor genes is
supported by numerous studies in which one or both of these two genes
have been found to be homozygously deleted in tumor cell lines and
primary tumors.15 Among the hematologic malignancies, p15
and p16 deletions have frequently been associated with T-acute lymphoblastic leukemia (T-ALL)17,18 and diffuse large
B-cell lymphomas.18,19 p16 deletion has also been reported
in a cell line derived from a diffuse large B-cell
lymphoma.19 However, its potential role in lymphoma
progression is unknown.
In the present study, we wished to determine whether loss of the CDK
inhibitor p16 could also be implicated in follicular lymphoma
progression. For our analysis, we used polymerase chain reaction
(PCR)-based microsatellite analysis combined with tissue microdissection for investigation of the deletional status of the 9p21
locus and immunohistochemistry to study the expression of the p16
protein.
PCR-based microsatellite analysis combined with tissue microdissection
has recently emerged as a powerful tool in performing loss of
heterozygosity (LOH) and gene deletion studies20 and offered several advantages to us. The critical microdissection step
allows one to enrich for tumor cells and, thereby, more accurately analyze tumors that have a high percentage of normal cells interspersed among the tumor cells. This is the case with many malignant lymphomas, and it is a problem that has previously prevented the accurate assessment of gene deletion in these tumors.17 Another
important advantage of PCR-based microsatellite analysis and
microdissection is that it can be applied to paraffin-embedded fixed
tissue samples, which are often the only form of archival biopsy
material available for genetic analysis. This is particularly true in
the case of progressed lymphomas, because the interval between the
occurrence of the low- and high-grade neoplasms is frequently many
years, and banked frozen tissue specimens from the paired biopsies are not frequently available.
In performing PCR-based microsatellite LOH studies on primary tumors,
homozygous deletions are interpreted by the apparent retention of
heterozygosity in one or more closely spaced microsatellite markers,
which must be flanked on both sides by other microsatellite markers
showing LOH.21,22 This apparent retention of heterozygosity is a result of the amplification of allele sequences contributed by
small numbers of contaminating normal cells inadvertently
microdissected along with neoplastic cells. This interpretation has
previously been validated by the demonstration of homozygous deletion
using Southern blot hybridization analysis and fluorescence in situ hybridization (FISH).21 Reed et
al22 have also confirmed this interpretation by the
demonstration of lack of immunohistochemical reactivity for p16 in head
and neck cancers with homozygous deletions detected by microsatellite
analysis.
To determine whether LOH or homozygous deletions at 9p21 involving p15
and p16 might be involved in the histologic progression of FCL to DLCL,
we studied 11 matched pairs of low-grade FCL (LGFCL) and their
progressed counterparts (DLCL), using microdissection and 10 microsatellite markers closely flanking these tumor-suppressor genes. A
comparative multiplex PCR assay was also used in the assessment of
homozygous deletions in this region, as previously described.23 In addition, immunohistochemical analysis for
p16 expression was performed and compared with the results of the genetic analyses.
Tumor Samples
Immunohistochemistry
Microdissection Technique
DNA Extraction
LOH Assays
Comparative Multiplex PCR
Genetic Analyses
Immunohistochemical Analyses p16.
All of the 9 evaluable LGFCLs showed (3+) reactivity (>75% of the
neoplastic cells) for p16 (Fig 5A). By
contrast, 3 of the 9 evaluable progressed DLCLs showed lack of p16
expression ( Correlation between genetic and immunohistochemical analyses.
All 9 LGFCLs showed retention of both (+/+) copies of chromosome 9p21
segments by microsatellite PCR analysis and were positive (3+) for p16
protein expression. All of the 5 progressed DLCLs with retention of one
or both copies of 9p21 segments showed (3+) reactivity for p16. Three
of the 4 progressed DLCLs with homozygous deletions of 9p21 that were
evaluable by immunohistochemistry showed complete lack of p16 protein
expression ( p53. p53 protein expression was detected in 3 of 11 (27%) LGFCLs and in 7 of 11 (64%) progressed DLCLs. Five of the 11 (45%) cases of progressed DLCL showed both homozygous 9p21 deletions and p53 overexpression. Four of the 9 progressed DLCL cases (44%) with lack of p16 protein expression showed p53 overexpression. Three of 9 (33%) LGFCL with (3+) p16 staining showed p53 overexpression, whereas 6 of 9 (67%) of the p16 protein positive LGFCL were negative for p53 protein.
About 90% of the deletions that involve p16 and p15 are homozygous
(particularly in hematologic malignancies) and often extend over 500 kb.18 These deletions generally include the entire interferon (IFN) gene cluster, the p16 locus, and the p15 locus, which
is located approximately 25 kb centromeric from the p16 locus. The
methylthioadenosine phosphorylase (MTAP) gene, which is located
approximately 100 kb telomeric to p16, is also frequently encompassed
by these deletions.18,24 The large size of these deletions
has suggested that a single deletional event may target multiple gene
loci and potentially lead to inactivation of several tumor-suppressor
genes. Indeed, the infrequent occurrence of p16 point mutations in
hematologic malignancies17,25 and other primary tumors with
hemizygous 9p deletions26,27 has led to suggestions that
p16 may not be the critical or only target of 9p
deletions.26 However, cytogenetic and molecular analyses have shown that, in primary hematolymphoid malignancies with
cytogenetic aberrations of 9p, the p16 locus is more frequently deleted
than the p15 locus.17,18,28 The smallest commonly deleted
region defined in leukemia-derived cell lines and primary
hematolymphoid tumors is an approximately 120-kb region bounded
centromerically by p15 and telomerically by the 3
Submitted August 4, 1997;
accepted February 3, 1998.
The authors thank Drs Michael Emmert-Buck and Zhengping Zhuang for their advice with regard to the microdissection technique.
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A. S. Baur, P. Shaw, N. Burri, F. Delacretaz, F. T. Bosman, and P. Chaubert Frequent Methylation Silencing of p15INK4b (MTS2) and p16INK4a (MTS1) in B-Cell and T-Cell Lymphomas Blood, September 1, 1999; 94(5): 1773 - 1781. [Abstract] [Full Text] [PDF]
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| Copyright © 1998 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
Abstract
Introduction
Abstract
3
), 10% to 25% as (
neoplastic large cells were dissected from the
DLCL biopsies (Fig 
-32P]dCTP (specific activity, 6,000 Ci/mmol), 10 mmol/L Tris-HCl (pH 8.3), 1.5 mmol/L MgCl2, 50 mmol/L KCl, 0.01% gelatin, and 0.25 U of AmpliTaq DNA polymerase
(Perkin Elmer Cetus, Norwalk, CT). The annealing temperatures used in
the various PCR reactions are as follows: IFNA and D9S171: 55°C;
D9S1747, D9S1748, D9S1749, and D9S1752: 58°C; D9S1751: 54°C;
and D9S144, D9S157, and D9S161: 56°C. PCR reactions were performed
over 30 to 35 cycles. An aliquot of each reaction mixture was diluted
with an equal volume of formamide loading dye (95% formamide, 20 mmol/L EDTA, 0.05% bromophenol blue, and 0.05% xylene cyanol).
Radiolabeled products were analyzed on a 6% sequencing gel, which was
then dried and autoradiographed. In pilot studies, we determined using
sensitivity assays that LOH could be easily scored when DNA extracts
were derived from microdissected samples with approximately 80%
neoplastic cells or greater (data not shown). In informative cases,
allelic loss was scored if the signal intensity from one allele was
significantly reduced in the tumor DNA when compared with the normal
DNA signal by direct visualization (Fig 
