56 research outputs found
Mouse RAD54 affects DNA double-strand break repair and sister chromatid exchange
Cells can achieve error-free repair of DNA double-strand breaks (DSBs) by homologous recombination through gene conversion with or without crossover. In contrast, an alternative homology-dependent DSB repair pathway, single-strand annealing (SSA), results in deletions. In this study, we analyzed the effect of mRAD54, a gene involved in homologous recombination, on the repair of a site-specific I-SceI-induced DSB located in a repeated DNA sequence in the genome of mouse embryonic stem cells. We used six isogenic cell lines differing solely in the orientation of the repeats. The combination of the three recombination-test substrates used discriminated among SSA, intrachromatid gene conversion, and sister chromatid gene conversion. DSB repair was most efficient for the substrate that allowed recovery of SSA events. Gene conversion with crossover, indistinguishable from long tract gene conversion, preferentially involved the sister chromatid rather than the repeat on the same chromatid. Comparing DSB repair in mRAD54 wild-type and knockout cells revealed direct evidence for a role of mRAD54 in DSB repair. The substrate measuring SSA showed an increased efficiency of DSB repair in the absence of mRAD54. The substrate measuring sister chromatid gene conversion showed a decrease in gene conversion with and without crossover. Consistent with this observation, DNA damage-induced sister chromatid exchange was reduced in mRAD54-deficient cells. Our results suggest that mRAD54 promotes gene conversion with predominant use of the sister chromatid as the repair template at the expense of error-prone SSA
Decreased PARP and procaspase-2 protein levels are associated with cellular drug resistance in childhood acute lymphoblastic leukemia
Drug resistance in childhood acute lymphoblastic leukemia (ALL) and acute
myeloid leukemia (AML) is associated with impaired ability to induce
apoptosis. To elucidate causes of apoptotic defects, we studied the
protein expression of Apaf-1, procaspases-2, -3, -6, -7, -8, -10, and
poly(adenosine diphosphate [ADP]-ribose) polymerase (PARP) in cells from
children with acute lymphoblastic leukemia (ALL; n = 43) and acute myeloid
leukemia (AML; n = 10). PARP expression was present in all B-lineage
samples, but absent in 4 of 15 T-lineage ALL samples and 3 of 10 AML
cases, which was not caused by genomic deletions. PARP expression was a
median 7-fold lower in T-lineage ALL (P < .001) and 10-fold lower in AML
(P < .001) compared with B-lineage ALL. PARP expression was 4-fold lower
in prednisolone, vincristine and L-asparaginase (PVA)-resistant compared
with PVA-sensitive ALL patients (P < .001). Procaspase-2 expression was
3-fold lower in T-lineage ALL (P = .022) and AML (P = .014) compared with
B-lineage ALL. In addition, procaspase-2 expression was 2-fold lower in
PVA-resistant compared to PVA-sensitive ALL patients (P = .042). No
relation between apoptotic protease-activating factor 1 (Apaf-1),
procaspases-3, -6, -7, -8, -10, and drug resistance was found. In
conclusion, low baseline expression of PARP and procaspase-2 is related to
cellular drug resistance in childhood acute lymphoblastic leukemia
Fusion of the homeobox gene HLXB9 and the ETV6 gene in infant acute myeloid leukemias with the t(7;12)(q36;p13)
Recently, we and others reported a recurrent t(7;12)(q36;p13) found in
myeloid malignancies in children < or =18 months of age and associated
with a poor prognosis. Fluorescence in situ hybridization studies mapped
the 12p13 breakpoint to the first intron of ETV6 and narrowed down the
region of 7q36 involved. By using the sequences made public recently by
the Human Genome Project, two candidate genes in 7q36 were identified: the
homeobox gene HLXB9 and c7orf3, a gene with unknown function. Reverse
transcription-PCR of two cases with t(7;12), using primers for c7orf3 and
ETV6, was negative. However, reverse transcription-PCR for HLXB9-ETV6
demonstrated alternative splicing; the two major bands corresponded to
fusion of exon 1 of HLXB9 to exons 2 and 3, respectively, of ETV6. The
reciprocal ETV6-HLXB9 transcript was not detected. It remains to be
elucidated if the leukemic phenotype is attributable to the formation of
the HLXB9-ETV6 fusion protein, which includes the helix-loop-helix and E26
transformation-specific DNA binding domains of ETV6 or to the disruption
of the normal ETV6 protein
Asparagine synthetase expression is linked with L-asparaginase resistance in TEL-AML1-negative but not TEL-AML1-positive pediatric acute lymphoblastic leukemia
Resistance to L-asparaginase in leukemic cells may be caused by an
elevated cellular expression of asparagine synthetase (AS). Previously, we
reported that high AS expression did not correlate to L-asparaginase
resistance in TEL-AML1-positive B-lineage acute lymphoblastic leukemia
(ALL). In the present study we confirmed this finding in TEL-AML1-positive
patients (n = 28) using microarrays. In contrast, 35
L-asparaginase-resistant TEL-AML1-negative B-lineage ALL patients had a
significant 3.5-fold higher AS expression than 43 sensitive patients (P <
.001). Using real-time quantitative polymerase chain reaction (RTQ-PCR),
this finding was confirmed in an independent group of 39 TEL-AML1-negative
B-lineage ALL patients (P = .03). High expression of AS was associated
with poor prognosis (4-year probability of disease-free survival [pDFS]
58% +/- 11%) compared with low expression (4-year pDFS 83% +/- 7%; P =
.009). We conclude that resistance to l-asparaginase and relapse risk are
associated with high expression of AS in TEL-AML1-negative but not
TEL-AML1-positive B-lineage ALL
Restricted 12p amplification and RAS mutation in human germ cell tumors of the adult testis
Human testicular germ-cell tumors of young adults (TGCTs), both seminomas
and nonseminomas, are characterized by 12p overrepresentation, mostly as
isochromosomes, of which the biological and clinical significance is still
unclear. A limited number of TGCTs has been identified with an additional
high-level amplification of a restricted region of 12p including the K-RAS
proto-oncogene. Here we show that the incidence of these restricted 12p
amplifications is approximately 8% in primary TGCTs. Within a single cell
formation of i(12p) and restricted 12p amplification is mutually
exclusive. The borders of the amplicons cluster in short regions, and the
amplicon was never found in the adjacent carcinoma in situ cells.
Seminomas with the restricted 12p amplification virtually lacked apoptosis
and the tumor cells showed prolonged in vitro survival like seminoma cells
with a mutated RAS gene. However, no differences in proliferation index
between these different groups of seminomas were found. Although patients
with a seminoma containing a homogeneous restricted 12p amplification
presented at a significantly younger age than those lacking it, the
presence of a restricted 12p amplification/RAS mutation did not predict
the stage of the disease at clinical presentation and the treatment
response of primary seminomas. In 55 primary and metastatic tumors from 44
different patients who failed cisplatinum-based chemotherapy, the
restricted 12p amplification and RAS mutations had the same incidence a
Prognostically useful gene-expression profiles in acute myeloid leukemia
BACKGROUND: In patients with acute myeloid leukemia (AML) a combination of
methods must be used to classify the disease, make therapeutic decisions,
and determine the prognosis. However, this combined approach provides
correct therapeutic and prognostic information in only 50 percent of
cases. METHODS: We determined the gene-expression profiles in samples of
peripheral blood or bone marrow from 285 patients with AML using
Affymetrix U133A GeneChips containing approximately 13,000 unique genes or
expression-signature tags. Data analyses were carried out with Omniviz,
significance analysis of microarrays, and prediction analysis of
microarrays software. Statistical analyses were performed to determine the
prognostic significance of cases of AML with specific molecular
signatures. RESULTS: Unsupervised cluster analyses identified 16 groups of
patients with AML on the basis of molecular signatures. We identified the
genes that defined these clusters and determined the minimal numbers of
genes needed to identify prognostically important clusters with a high
degree of accuracy. The clustering was driven by the presence of
chromosomal lesions (e.g., t(8;21), t(15;17), and inv(16)), particular
genetic mutations (CEBPA), and abnormal oncogene expression (EVI1). We
identified several novel clusters, some consisting of specimens with
normal karyotypes. A unique cluster with a distinctive gene-expression
signature included cases of AML with a poor treatment outcome.
CONCLUSIONS: Gene-expression profiling allows a comprehensive
classification of AML that includes previously identified genetically
defined subgroups and a novel cluster with an adverse prognosis
The structure-specific endonuclease Ercc1-Xpf is required to resolve DNA insterstrand cross-link-induced double-strand breaks
Interstrand cross-links (ICLs) are an extremely toxic class of DNA damage incurred during normal metabolism or cancer chemotherapy. ICLs covalently tether both strands of duplex DNA, preventing the strand unwinding that is essential for polymerase access. The mechanism of ICL repair in mammalian cells is poorly understood. However, genetic data implicate the Ercc1-Xpf endonuclease and proteins required for homologous recombination-mediated double-strand break (DSB) repair. To examine the role of Ercc1-Xpf in ICL repair, we monitored the phosphorylation of histone variant H2AX (gamma-H2AX). The phosphoprotein accumulates at DSBs, forming foci that can be detected by immunostaining. Treatment of wild-type cells with mitomycin C (MMC) induced gamma-H2AX foci and increased the amount of DSBs detected by pulsed-field gel electrophoresis. Surprisingly, gamma-H2AX foci were also induced in Ercc1(-/-) cells by MMC treatment. Thus, DSBs occur after cross-link damage via an Ercc1-independent mechanism. Instead, ICL-induced DSB formation required cell cycle progression into S phase, suggesting that DSBs are an intermediate of ICL repair that form during DNA replication. In Ercc1(-/-) cells, MMC-induced gamma-H2AX foci persisted at least 48 h longer than in wild-type cells, demonstrating that Ercc1 is required for the resolution of cross-link-induced DSBs. MMC triggered sister chromatid exchanges in wild-type cells but chromatid fusions in Ercc1(-/-) and Xpf mutant cells, indicating that in their absence, repair of DSBs is prevented. Collectively, these data support a role for Ercc1-Xpf in processing ICL-induced DSBs so that these cytotoxic intermediates can be repaired by homologous recombination
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