Human chronic lymphocytic leukemia B cells can escape DNA damage-induced apoptosis through the nonhomologous end-joining DNA repair pathway

doi:10.1182/blood-2004-07-2888

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Blood, 15 June 2005, Vol. 105, No. 12, pp. 4776-4783.
Prepublished online as a Blood First Edition Paper on February 17, 2005; DOI 10.1182/blood-2004-07-2888.

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NEOPLASIA
Human chronic lymphocytic leukemia B cells can escape DNA damage-induced apoptosis through the nonhomologous end-joining DNA repair pathway
Ludovic Deriano, Olivier Guipaud, Hélène Merle-Béral, Jacques-Louis Binet, Michelle Ricoul, Gaby Potocki-Veronese, Vincent Favaudon, Zofia Maciorowski, Catherine Muller, Bernard Salles, Laure Sabatier, and Jozo Delic
From the Laboratoire de Radiobiologie et Oncologie, Commissariat à l'Enegie Atomique, Fontenay-aux-Roses, France; the Département d'Hématologie, Unité Claude Bernard C20, Hôpital Pitié-Salpêtrière, Paris, France; Institut Curie, Section de Recherche (Institut National de la Santé et de la Recherche Médicale [INSERM] U612), Centre Universitaire, Orsay Cedex and Laboratoire de Cytométrie, Section Médicale, Paris, France; and the Institut de Pharmacologie et de Biologie Structurale (Centre National de la Recherche Scientifique [CNRS] Unité Propre de Recherche [UPR] 9062), Toulouse, France.

   Abstract

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Nonhomologous end-joining (NHEJ) DNA factors maintain genomicstability through their DNA double-strand break (DSB) repairand telomere-associated activities. Unrepaired or misrepairedDSBs can lead to apoptotic death or chromosomal damage. TheB cells of some B-chronic lymphocytic leukemia (B-CLL) patientsare resistant to radiation-induced apoptosis in vitro. We showhere that the novel DNA-dependent protein kinase (DNA-PK) inhibitor,NU7026 (2-(morpholin-4-yl)-benzo[h]chomen-4-one), and the phosphatidylinositol3 (PI-3) kinase inhibitor, wortmannin, restored sensitivityto DNA damage-induced apoptosis of otherwise resistant cells.These resistant malignant B cells also escaped DSB-induced apoptosisfollowing exposure to etoposide or neocarzinostatin. We foundthat at 15 minutes after irradiation, the levels of NHEJ (asmeasured by an in vitro DSB end-ligation assay) and DNA-PK catalyticsubunit (DNA-PKcs) activity were, respectively, 2-fold and 4-foldhigher in radio-resistant than in radio-sensitive B-CLL cellsor Epstein-Barr virus (EBV)-transformed B cells. Ku70/Ku80 heterodimerDNA end-binding activity was also 2- to 3-fold higher in theresistant B-CLL cell subset compared with the sensitive B-CLLcell subset. Our results provide the first evidence that overactivatingthe NHEJ DNA repair pathway impairs DNA damage-induced apoptosisin malignant B cells and that this may contribute to their resistanceto current chemotherapy. (Blood. 2005;105:4776-4783)

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Mammalian cells respond to a variety of genotoxic stresses,including exposure to ionizing radiation and topoisomerase inhibitors,and endogenous reactive oxygen species, via 2 mechanisms formaintaining genome integrity: DNA repair and apoptosis. Inaccuraterepair or a lack of repair of double-strand breaks (DSBs) canlead to apoptosis¹ or to mutations or large-scale genomic instabilitythrough the generation of nonlethal chromosomal aberrations.²
DSBs are repaired by homologous recombination (HR) and by nonhomologousend-joining (NHEJ). NHEJ is the predominant mechanism in highereukaryotes, whereas single-celled organisms (such as yeast)rely more heavily on HR. DNA-dependent protein kinase (DNA-PK)is a key component of the NHEJ pathway.³ DNA-PK is a nuclearserine/threonine protein kinase, comprising a 460-kDa catalyticsubunit, DNA-PKcs, and a DNA-binding subunit, the Ku autoantigen(a Ku70 and Ku80 protein dimer). The Ku70/Ku80 heterodimer bindsthe free DNA ends generated by DSBs and recruits the catalyticsubunit of the complex.^4-6 In vitro, this active DNA-PK complexcan phosphorylate many DNA-bound proteins including protein53 (p53), Ku, X-ray cross-complementing group 4 (XRCC4), andDNA-PKcs^3,7,8 and can bind to XRCC4 and ligase IV, which jointogether the ends of the broken DNA strands.^8-10
Little is known about the role of the NHEJ repair pathway inapoptosis. Studies suggesting that DNA-PK plays a role in apoptosisremain controversial and principally relate to the interactionof this protein with p53.¹¹ The results from some studies indicatethat DNA-PK activates and phosphorylates p53^12,13 and murinedouble mutant 2 (MDM2)¹⁴ after DNA damage. However, other groupsreported that DNA-PKcs-defective mice and DNA-PKcs-defectivecell lines display normal p53-mediated apoptosis responses.^15,16DNA-PK activity has been implicated in resistance to nitrogenmustard therapy in leukemia cells,^17,18 but further studiesare necessary to understand how these cells escape apoptosisafter this genotoxic stress.
We investigated this phenomenon using lymphocytes from patientswith B-chronic lymphocytic leukemia (B-CLL), a disease characterizedby the accumulation of mature-looking malignant B cells in theperipheral blood, bone marrow, and lymph nodes.¹⁹ B-CLL cellsalso display both chromosomal instability and defects in apoptoticcell death. We investigated whether the NHEJ DNA repair systemprevents apoptosis in response to DNA damage in these cells.We reported previously that some B-CLL patients' B cells arecompletely resistant to radiation-induced apoptosis.^20,21 DNAdamage is repaired more rapidly in these resistant cells thanin sensitive B-CLL cells, but more chromosomal aberrations accumulatein the resistant cells after the first cell division.²²
We show here that B-CLL cells resistant to ${gamma}$ -radiation-inducedapoptosis are also completely resistant to apoptosis inducedby neocarzinostatin (NCS) and etoposide VP-16 (4'-demethyl-epipodophyllotoxin-9-[4,6-O-ethylidene- ${beta}$ -D-glucopyranoside]),compounds that specifically cause DNA DSBs. Treatment of theseresistant cells with the DNA-PKcs-specific inhibitor, NU7026(2-(morpholin-4-yl)-benzo[h]chomen-4-one),^23-25 or with thephosphatidylinositol 3 (PI-3) kinase inhibitor, wortmannin,^26,27led to them undergo apoptosis after DNA damage. In vitro NHEJassay for DSB end-ligation revealed that end-ligation efficiencywas 2-fold higher in resistant B-CLL cells than in sensitiveB-CLL cells or in Epstein-Barr virus (EBV)-transformed B lymphocytesat 15 minutes after irradiation (10 Gy). This alteration inNHEJ activity after DNA damage correlated with our findingsthat DNA-PKcs activity was 4-fold higher 15 minutes after irradiationand that Ku70/80 heterodimer DNA end-binding (DEB) activitywas constitutively 2- to 3-fold higher in the resistant cells.This is the first time that a deregulated DNA repair systemhas been shown to allow human malignant cells to escape apoptosisafter DNA damage. These results should improve current understandingof cancer cell resistance to genotoxic chemotherapy.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patients, isolation of B-CLL lymphocytes, and cell culture
The patients enrolled in the study were diagnosed with B-CLLfollowing cytologic and immunologic analyses and followed-upat the Pitié-SalpêtrièreHospital (Paris,France) between 1998 and 2004. Approval for these studies wasobtained from the institutional review boards of the Commissariatà l'Energie Atomique and the Hospital Pitié-Salpêtrièrein Paris. All patients gave informed consent. B lymphocyteswere purified and maintained in culture as previously described.^20,21The MO59J, MO59K,²⁸ CHO-K1, and xrs6 cell lines²⁹ were grownin Dulbecco modified Eagle medium (DMEM; Invitrogen, Cergy Pointoise,France) supplemented with 10% fetal calf serum (D. Dutscher,France) and an antibiotic-antimycotic cocktail (Invitrogen).The EBV-transformed B-lymphocyte cell line was grown in RPMI1640 medium supplemented with 10% heat-inactivated fetal calfserum.
Irradiation and cell treatments
Purified B-CLL lymphocytes were irradiated as previously described.³⁰Drugs were then added directly to the cell culture medium atthe concentrations indicated. Neocarzinostatin was preparedand titrated as described.³¹ Working solutions were preparedimmediately before use in cold 0.01 M sodium phosphate buffer(pH 6.6). VP-16, okadaic acid, NU7026 (Calbiochem, Fontenay-Sous-Bois,France), and wortmannin (Sigma, Saint Quentan Fallavier, France)were prepared in dry dimethyl sulfoxide and stored at -20°C.Equal volumes of the solvents or buffers used were added tountreated cell cultures as controls. To determine the effectof NU7026 and wortmannin on irradiation-induced apoptosis, cellswere pretreated with either 10 µM NU7026 for one houror 1 µM wortmannin for 30 minutes, washed twice in phosphate-bufferedsaline (PBS), and irradiated at 10 Gy. Cells were then culturedin medium containing either 10 µM NU7026 or 1 µMwortmannin, and the number of apoptotic cells was then countedas described in the next paragraph.
Apoptotic cell counts: B-CLL cell classification according to sensitivity to ${gamma}$ -radiation-induced apoptosis
After 24 hours of cell culture with or without the various drugtreatments, the number of cells with chromatin-associated fluorescenceand characteristic apoptotic morphology (ie, chromatin condensationand nuclear fragmentation) was counted as previously described.³⁰B-CLL cells were then classified into 2 groups depending ontheir sensitivity to ${gamma}$ -irradiation-induced apoptosis. B lymphocyteswith postirradiation apoptosis scores identical to those ofuntreated cells (spontaneous apoptosis generally occurs in <20% of untreated cells) were classified as the resistant subset(R), and B lymphocytes with an apoptosis score of more than40% were classified as the sensitive subset (S). Approximately15% of B-CLL patients produce B cells that are completely resistantto radiation-induced apoptosis, and so far B cells from 225B-CLL patients have been tested for their sensitivity to radiation-inducedapoptosis in vitro.
Preparation of in vitro cell-free extracts and DSB end-ligation assay ("NHEJ activity assay")
In vitro cell-free extracts and DSB end-ligation assays wereprepared and carried out as described previously.³²
Cell-free extracts
B-CLL extracts (0.15-0.2 mL) with a protein concentration ofbetween 5 and 10 mg/mL were prepared from approximately 1 x10⁹ B-CLL lymphocytes. MO59J, MO59K, and EBV-transformed B-cellextracts (0.3-0.8 mL) were prepared from 5 x 10⁸ cells and hadprotein concentrations of between 7 and 10 mg/mL. Extracts werestored as 20-µL aliquots in liquid nitrogen and remainedactive for 6 to 12 months. Before being measured for NHEJ activity,extracts were dialyzed against freshly prepared M-buffer (50mM 3-(N-morpholino)-2-hydroxy-propane sulfonic acid [MOPSO]-NaOH[pH 7.5], 40 mM KCl, 10 mM MgCl₂, 5 mM 2-mercaptoethanol) for30 minutes at 4°C using microdialysis filters (0.025-µmpore diameter; Millipore, Molsheim, France).
DNA substrates
The 2 substrates for 5'-cohesive end-ligation were derived frompSP65 and pUC18 (2.69 kb; Sigma) after linearization of the2 vectors by digestion with BamHI and EcoRI (New England Biolabs,Beverly, MA), respectively. Similar results were obtained withboth DNA substrates (data not shown). Substrates were recoveredfrom gels using a gel extraction kit (Qiagen, Courtabeuf, France).
NHEJ assay and analysis of the products
Preliminary experiments revealed that ligation and NHEJ werecomplete for both the cell line and B-CLL lymphocyte extractsafter incubation for 3 hours at 25°C. For standard reactions,10 ng linearized plasmid (1 µL) was incubated in a totalvolume of 10 µL reaction medium containing 40 µgprotein extract (8 µL) in M-buffer (pH 7.5) supplementedwith 1 mM adenosine triphosphate (ATP), 200 µM deoxynucleosidetriphosphate (dNTPs) (50 µM of each nucleotide), and 50ng/µL bovine serum albumin. Where indicated, protein sampleswere pretreated with wortmannin (1 µM) or NU7026 (10 µM)for 20 minutes on ice before being assayed for end-joining activity.Reactions were stopped by adding a solution containing 20 mMTris (tris(hydroxymethyl)aminomethane)-HCL (pH 7.5), 10 mM EDTA(ethylenediaminetetraacetic acid), 1% sodium dodecyl sulfate(SDS) and incubating at 65°C for 5 minutes. Samples werethen digested with 2 mg/mL proteinase K for 30 minutes at 37°C.The equivalent of 2 ng DNA substrate was subjected to electrophoresisin 1% agarose gels containing 1 µg/mL ethidium bromidefollowed by Southern blot analysis using a pSP65- or PUC18-specificprobe labeled with [ ${alpha}$ -³²P] deoxycytidine triphosphate (dCTP)by random priming (random labeling kit; Roche Diagnostics, Meylan,France). Reaction products were quantified by phosphor imaging(Storm 860 and ImageQuant software; Amersham-Pharmacia Biotech,Orsay, France). End-ligation activity was assessed by measuringthe conversion of monomeric plasmids to ligated products. Ligationefficiency was calculated by dividing the densitometry readingsfor the sum of all converted plasmid products by those for thesum of all products. The changes in NHEJ activity after treatmentof B cells with 10 Gy ${gamma}$ -irradiation were calculated by dividingthe ligation efficiency of B-cell extracts exposed to irradiationfor 15 minutes by the ligation efficiency of untreated controlB cells.
DNA-PKcs activity
DNA-PK "pull-down" kinase assays were performed as previouslydescribed.³³ Nuclear extracts were prepared as follows: at theindicated time points after irradiation, 1 x 10⁷ B-CLL lymphocyteswere washed twice in PBS and lysed by incubation in 200 µLice-cold hypotonic buffer (1.5 mM MgCl₂, 5 mM KCl, 10 mM HEPES[pH 7.5], 5 mM EDTA, 1 mM phenylmethylsulfonyl fluoride [PMSF],Mini-Complete protease inhibitor cocktail [Roche Diagnostics],and 0.5% nonidet P-40). After centrifugation (5000g, 10 minutes,4°C), the pellet containing cell nuclei was recovered andsuspended in 100 µL modified buffer (50 mM NaF, 20 mMHepes [pH 7.5], 450 mM NaCl, 25% glycerol, 0.2 mM EDTA, 0.5mM 1,4-dithiothreitol [DTT], 0.5 mM PMSF, and Mini-Completeprotease inhibitor cocktail) as described previously for whole-cellextracts.³³ The nuclear suspension was then frozen at -70°Cand thawed at 30°C 3 times. After centrifugation (10 000g,10 minutes, 4°C), supernatants were recovered and storedat -80°C until use. Protein concentration was determinedby the Bradford method. Where indicated, protein samples werepretreated with wortmannin (1 µM) or NU7026 (10 µM)before being used in DNA-PKcs assays. Samples were assayed inthe presence either of a native (EPPLSQEAFADLWKK; Promega, Sarl,France) or of a mutant (EPPLSEQAFADLWKK; negative control) peptidederived from p53. Radiolabeled, phosphorylated substrate wassubjected to tricine SDS-polyacrylamide gel electrophoresis(PAGE, 18% gels). [ ${gamma}$ -³²P] ATP incorporation into the substratepeptide was quantified using the Storm 860 and ImageQuant software(Amersham-Pharmacia Biotech). The MO59J and MO59K cell lineswere used as controls.
Ku heterodimer DEB activity
Whole-cell extracts were prepared from B-CLL lymphocytes usingthe modified buffer used to make the nuclear extracts for theDNA-PK pull-down assays. The double-stranded 18-mer nucleotide(5'GATCTAGCTGCACCGGAC3',5'GTCCGGTGCAGCTAGATC3') was used toexamine Ku DNA-end binding. Electrophoretic mobility shift assays(EMSAs) were performed as previously described,¹⁸ with the exceptionthat electrophoresis conditions were modified to enable us todetect supershifts (6% acrylamide gels and 0.25X Tris-borate-EDTA[TBE] running buffer). Extracts from the CHO-K1, xrs6, MO59K,and MO59J cell lines were used as controls. Supershifts wereperformed using a polyclonal Ku70 antibody (Santa Cruz Biotechnology,Santa Cruz, CA) at a 1:10 dilution. Immunodepletion studieswere performed by incubating 5 µg B-CLL cell extract with125 ng or 250 ng monoclonal Ku70 antibody (Ab4; Neomarkers,Fremont, CA) for one hour at 4°C on a rotary wheel. Extractswere then incubated for a further 2 hours at 4°C with proteinA-Sepharose (Amersham-Pharmacia Biotech). After centrifugation(5 minutes at 4°C, 13 000 rpm), the supernatant was assayedfor Ku heterodimer DEB activity and subjected to Western blotanalysis.

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Figure 1.. B-CLL cell sensitivity to DSB-induced apoptosis. R indicates resistant B-CLL cells; and S, sensitive B-CLL cells. (A) Sensitivity of B-CLL cells to ${gamma}$ -irradiation-induced apoptosis (R: n = 13 samples; S: n = 79 samples). Sensitivity of R (n = 5 samples) and S (n = 15 samples) B-CLL cells to NCS-induced (B), VP16-induced (C), and okadaic acid-induced (D) apoptosis. Percentages of apoptotic cells are the means (± SEM) of duplicate experiments on B-CLL samples.

Western blot
Protein extracts were analyzed by Western blotting as previouslydescribed.³⁴ Proteins were detected using Ku70 (Ab-4, cloneN3H10), Ku80 (Ab-2, clone 111), Ku80 variant form (Ab-7, cloneS10B1; Neomarkers), and DNA-PKcs (ab230; Abcam, Cambridge, UnitedKingdom) antibodies at dilutions of 1:10 000, 1:5000, 1:200,and 1:5000, respectively. The XRCC4 antibody (ab145; Abcam)was used at a dilution of 1:2000 and the ligase IV antibodywas used at a dilution of 1:500 (a gift from Tomas Lindahl,Imperial Cancer Research Fund [ICRF], United Kingdom).

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
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A B-CLL cell subset is specifically resistant to DSB-induced apoptosis
B cells from most B-CLL patients underwent apoptosis within24 hours of ${gamma}$ -irradiation, whereas B cells from some patientsdid not (Figure 1A). Of 92 independent B-CLL cell samples, 13were totally resistant to apoptosis induced by exposure to 10Gy irradiation (mean ± SEM percentage of cells in thissubset undergoing spontaneous apoptosis: 10.7% ± 6.2%,whereas those undergoing 10 Gy ${gamma}$ -ray-induced apoptosis: 19.5%± 8%). More than 40% of the cells in the remaining 79samples underwent apoptosis after exposure to only 2 Gy ${gamma}$ -irradiation(15.8% ± 7.3% underwent spontaneous apoptosis, 42.7%± 11.3% underwent apoptosis after exposure to 2 Gy, and62.5% ± 12.3% underwent apoptosis after exposure to 10Gy). We investigated whether the difference in sensitivity toirradiation-induced apoptosis between these 2 B-CLL cell subsetswas associated with the level of DSB injury. We used the radiomimeticcompound NCS. NCS cleaves DNA during the course of a reactionthat leads to complete degradation of the drug after a few minutes.³⁵As found previously for ${gamma}$ -ray dose,³⁶ the incidence of DSB increasedlinearly with NCS concentration; 1 nM NCS lead to the same amountof DSBs as 1.21 Gy ${gamma}$ -rays.³⁷ We studied the sensitivity of 5representative resistant (in which 9.7% ± 2% of cellsunderwent spontaneous apoptosis and 14.7% ± 2.8% underwentapoptosis after exposure to 10 Gy ${gamma}$ -rays; data not shown) and15 representative sensitive (in which 19.7% ± 8.8% ofcells underwent spontaneous apoptosis and 74.8% ± 14.1%of cells underwent apoptosis after exposure to 10 Gy of ${gamma}$ -rays;data not shown) B-CLL samples to increasing concentrations ofNCS (Figure 1B). Radio-resistant B-CLL samples were also resistantto NCS-induced apoptosis (11.9% ± 4.0% of cells underwentspontaneous apoptosis and 20.2% ± 8.0% underwent 8 nMNCS-induced apoptosis). In the sensitive subset, 1.65 nM NCS(yielding the same number of DSBs as 2 Gy ${gamma}$ -rays) induced apoptosisin 45% plus or minus 17% of cells (Figure 1B) and 2 Gy ${gamma}$ -raysinduced apoptosis in 42.7% plus or minus 11.3% of cells (Figure 1A).We then studied the sensitivity of the same 5 resistantand 15 sensitive B-CLL samples to VP-16 (Figure 1C). VP-16 causesDSBs by inhibiting topoisomerase II and is used in cancer chemotherapy.³⁸As with NCS, radio-resistant B-CLL cells were also resistantto VP-16-induced apoptosis (13.6% ± 6.6% of cells underwentspontaneous apoptosis and 23.6% ± 9.9% of cells underwentapoptosis induced by 20 µM VP16). Radio-sensitive B-CLLcells were also sensitive to VP-16-induced apoptosis (20.0%± 9.2% of cells underwent spontaneous apoptosis and 69.3%± 7.7% underwent apoptosis induced by 20 µM VP16).The protein phosphatase inhibitor, okadaic acid (OA), has beenshown previously to induce apoptosis in B-CLL cells.³⁹ Thisinhibitor induced apoptosis in both the radio-resistant andradiosensitive B-CLL samples. The percentage apoptosis did notdiffer significantly between the 2 cell types at any of theconcentrations tested (0-100 nM OA). These results indicatethat the OA-induced cell death pathway is fully functional inboth types of B-CLL cells (Figure 1D).

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Figure 2.. The PI-3 kinase inhibitor wortmannin and the DNA-PKcs inhibitor NU7026 sensitize resistant B-CLL cells to ${gamma}$ -irradiation-induced apoptosis. R indicates resistant B-CLL (n = 5 samples); and S, sensitive B-CLL (n = 7 samples). (A) B-CLL cells were either left untreated (NT) or treated with 1 µM wortmannin alone (WM), with 10 Gy irradiation alone (IR) or with 1 µM wortmannin and 10 Gy irradiation (IR+WM). (B) B-CLL cells were either left untreated (NT) or treated with 10 µM NU7026 alone (NU7026), with 10 Gy irradiation alone (IR), or with 10 µM NU7026 and 10 Gy irradiation (IR+NU7026). Percentages of apoptotic cells are means (± SEM) of duplicate experiments on n B-CLL samples.

Inhibition of DNA-PKcs by NU7026 and wortmannin restores the sensitivity of resistant B-CLL cells to irradiation-induced apoptosis
We hypothesized that the NHEJ pathway was responsible for theresistance of some B-CLL cells to DSB-induced apoptosis. Totest this hypothesis, we used 2 DNA-PK inhibitors: NU7026, whichat low concentrations inhibits DNA-PKcs (median inhibitory concentration[IC50] = 0.23 µM) but not PI-3 kinase, ATM, and ATR (IC50= 13 µM, IC50 > 100 µM, and IC50 > 100 µM,respectively),²⁴ and wortmannin, which inhibits all PI-3 kinasesand PI-3-like kinases, including DNA-PKcs.²⁷ The resistanceof some B-CLL cells to irradiation-induced apoptosis was nearlyabolished by inhibiting DNA-PK (Figure 2). The number of apoptoticcells was higher for ${gamma}$ -irradiated (10 Gy) resistant B-CLL cellstreated with 1 µM wortmannin (53.3 ± 14.3%) thanfor cells treated with irradiation alone (14.7 ± 8.1%)(Figure 2A). NU7026 also restored the sensitivity of resistantB-CLL cells to radiation-induced apoptosis (Figure 2B): thenumber of apoptotic cells was significantly higher for ${gamma}$ -irradiated(10 Gy) resistant B cells treated with 10 µM NU7026 (45.7± 9.1%) than for resistant cells treated with irradiationalone (13.7 ± 6.4%). NU7026 and wortmannin had no significanteffect on percentage apoptosis in ${gamma}$ -irradiated sensitive B-CLLcells (Figure 2A-B). In addition, wortmannin and NU7026 inhibitedNHEJ-mediated DNA repair and DNA-PKcs phosphorylation in boththe sensitive and resistant B-CLL cells (Figures 3C, 4D).
NHEJ is overactivated after DNA damage in resistant B-CLL cells
We performed the DSB end-ligation assay to measure NHEJ activityin 3 sensitive and 3 resistant B-CLL cell extracts. These sampleswere representative of the 2 B-CLL cell subsets, and, with theexception of one resistant sample displaying p53 dysfunctionand carrying a mutation at position 220 (Y $->$ A; data not shown),all the samples used produced wild-type p53. The ligation efficienciesof resistant and sensitive B-CLL cell extracts were comparedwith those of an EBV-transformed B-cell line (B cells). Measurementswere taken before and 15 minutes after exposure to 10 Gy ${gamma}$ -irradiation.All experiments were performed at 25°C with 40 µgprotein extract, and reactions were allowed to continue for3 hours (linear phase of the end-ligation reaction under conditionswhere all monomers are not converted to ligation products; datanot shown). We found that NU7026 and wortmannin inhibited DNArepair in both untreated and irradiated extracts from resistantand sensitive B-CLL cells (Figure 3C), indicating that DSB end-ligationactivity was completely dependent on DNA-PK activity. Moreover,DSB endligation activity was detected in extracts from MO59K(DNA-PKcs proficient) cells but not in extracts from MO59J (DNA-PKcsdeficient) cells, demonstrating that the DNA repair is a DNA-PKcs-dependentNHEJ process (Figure 3D). We found that the efficiency of NHEJrepair increased by 2-fold (2.36 ± 0.23) in the resistantB-CLL cells after exposure to 10 Gy irradiation, whereas noincrease after irradiation was detected in sensitive B-CLL cellsor EBV-transformed B lymphocytes (1.07 ± 0.1 and 1.03± 0.15 respectively, Figure 3A and 3B). Experiments weredone in duplicate with 3 different resistant and 3 differentsensitive B-CLL samples; smallest and highest values calculatedwith resistant samples were, respectively, 2.01 and 2.64, whereassmallest and highest values calculated with sensitive B-CLLsamples were, respectively, 0.94 and 1.24, indicating that onlysmall variations appeared between patient samples of each group.However, as there is a relatively small number of samples, thevariation shown in Figure 3 (2-fold increase in resistant cells)may not reflect that seen in a larger population. Western blotanalysis of extracts from resistant and sensitive B-CLL cellsrevealed no significant differences in DNA-PKcs, Ku80, and Ku70levels, before or after irradiation (Figure 5E). Although wefound that the levels of both XRCC4 and ligase IV may be slightlyhigher in 3 resistant than in 3 sensitive B-cell samples, bothbefore and after irradiation (Figure 5E), experiments done ona larger series of samples (6 resistant and 7 sensitive) revealedthat XRCC4 and ligase IV expression varied between samples andthat, overall, resistant B-CLL cell samples did not producehigher amounts of these proteins than sensitive samples (datanot shown). The Ku70 and Ku80 levels were similar in all thecell samples tested (data not shown).

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Figure 3.. NHEJ DNA repair pathway is overactivated in resistant B-CLL cells after DNA damage. (A) NHEJ activity in untreated cells (Irradiation -) and cells exposed to 10 Gy irradiation (Irradiation +). Assays were carried out using a resistant B-CLL lymphocyte extract (R), a sensitive B-CLL cell extract (S), and an EBV-transformed B-lymphocyte extract (B cells). The results shown are representative of those obtained with all the cell extracts tested (n = 3 for resistant B-CLL samples, n = 3 for sensitive B-CLL samples, and n = 3 for EBV-transformed B-cell samples). (B) Changes in NHEJ activity after exposure to 10 Gy irradiation were calculated from the mean (± SEM) activities recorded in duplicate experiments on 3 different resistant B-CLL cell extracts (R), 3 different sensitive B-CLL cell extracts (S), and 3 different EBV-transformed B-lymphocyte extracts (B cells). (C) NHEJ activity in cells that were either left untreated (-) or treated (+) with 10 Gy irradiation, 1 µM wortmannin, or 10 µM NU7026. Assays were performed on resistant B-CLL cell extracts (R) and sensitive B-CLL cell extracts (S). A representative experiment is shown. (D) NHEJ activity assay with DNA-PKcs-deficient cell line extract (MO59J) and wild-type cell line extract (MO59K). A representative experiment is shown. See Supplemental Figure S1 for more information.

Early activation of DNA-PKcs in resistant but not sensitive B-CLL cell samples in response to ${gamma}$ -irradiation
We investigated whether the increase in NHEJ DNA repair efficiencyin resistant cells was related to an alteration in DNA-PKcsactivity. A "pull-down" assay³³ was performed before and atdifferent times after irradiation in 3 resistant and 3 sensitiveB-CLL cell extracts. DNA-PKcs kinase activity was determinedby measuring phosphorylation of a peptide substrate derivedfrom wild-type p53. The radioactivity associated with the mutatedpeptide did not exceed 6% of that associated with the substratepeptide (data not shown). Furthermore, no phosphorylation ofthe wild-type p53-derived substrate was detected in extractsfrom the DNA-PKcs-deficient MO59J cell line, indicating thatphosphorylation of the wild-type substrate is a result of DNA-PKcsactivity, rather than of other protein kinases (Figure 4B).We found that DNA-PKcs kinase activity was slightly higher innuclear protein extracts from resistant than from sensitiveB-CLL samples before irradiation treatment (Figure 4A-C). Asexpected, wortmannin and NU7026 completely inhibited DNA-PKcsactivity in both the sensitive and resistant B-CLL cells (Figure 4D).At 15 minutes after irradiation, kinase activity was 4-foldhigher in the resistant B-CLL cells than in the sensitive B-CLLcells (Figure 4A,C). The kinase activity in the resistant cellsremained 3- to 3.5-fold higher than in sensitive cells at 60and 150 minutes after irradiation (Figure 4C). This increasein kinase activity was completely abolished by treatment ofthe resistant cells with NU7026 and wortmannin (Figure 4D).

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Figure 4.. Early increases in DNA-PKcs activity in resistant B-CLL cell extracts after ${gamma}$ -irradiation. (A) DNA-PKcs activity in resistant B-CLL (R) nuclear protein extracts (25 µg/lane) and sensitive B-CLL (S) nuclear protein extracts (25 µg/lane) at the indicated times after treatment with 10 Gy ${gamma}$ -irradiation. The results shown are representative of those obtained in all extracts tested (n = 3 for resistant samples and n = 3 for sensitive samples). (B) DNA-PKcs activity in untreated nuclear protein extracts from 3 resistant B-CLL samples (R₁,R₂,R₃) and from 3 sensitive B-CLL samples (S₁,S₂,S₃). (C) Mean (± SEM) DNA-PKcs activity in 3 resistant B-CLL samples (R) and 3 sensitive B-CLL samples (S) at the indicated times after irradiation. Values are given in arbitrary units (AU). (D) DNA-PKcs activity in resistant (R) and sensitive (S) B-CLL nuclear protein extracts (25 µg/lane) from cells that were either left untreated (-) or treated with 10 Gy irradiation (+, measurements were carried out 15 minutes after irradiation), 1 µM wortmannin, or 10 µM NU7026. A representative experiment is shown. See Supplemental Figure S2 for more information.

Regulation of DNA-PK activity: increased Ku70/80 heterodimer DNA-binding activity in resistant B-CLL cells
The DNA end-binding activity of the Ku70/80 heterodimer is thefirst limiting step in the formation of an active DNA-PK complex.Thus, the increase in DNA-PK activity in the resistant B-CLLsamples may be associated with an increase in Ku heterodimerDEB activity. We therefore tested this possibility using the3 resistant and 3 sensitive B-CLL samples described earlier.EMSA was performed to assess binding of the Ku heterodimer complexto radiolabeled double-stranded DNA.¹⁸ Assays were carried outin the presence of a circular plasmid (competitive substrate),and shifts in mobility were detected by autoradiography (Figure 5A).The following lines of evidence indicate that the band-shiftsobserved corresponded to binding of the Ku70/Ku80 heterodimerDNA complex to the double-stranded DNA: (1) the band-shift wasnot observed following immunodepletion of Ku70 (Figure 5D lanes1-3), (2) a supershift was observed after the addition of anti-Ku70antibodies (Figure 5D lanes 4-5), and (3) the complex was notdetected in extracts from xrs6 cells, expressing a mutated formof Ku80, but was detected in extracts from CHO-K1 control cells(Figure 5C). We also noticed that both MO59J and MO59K cellshad functional Ku heterodimer DNA end-binding activity (Figure 5C).The Ku DEB activity was quantified in 3 resistant and 3sensitive B-CLL samples, before and at various times followingirradiation. Unlike DNA-PKcs activity, Ku DEB activity was significantlyhigher (2- to 3-fold) in resistant B-CLL samples than in sensitiveB-CLL samples, both before and after ${gamma}$ -irradiation (Figure 5B).Differences in Ku DEB activity between the resistant and sensitiveB-CLL samples were not caused by differences in the level ofexpression of the Ku70 and Ku80 proteins (Figure 5E). Previousstudies have reported that a variant form of Ku80 (estimatedmolecular weight [MW] = 69 kDa) may be expressed in cells withlow DNA-PK activity.¹⁸ Although the Ku70/Ku80 variant heterodimerbinds to DNA ends, it has a decreased ability to recruit thecatalytic subunit, DNA-PKcs.^18,40 Western blot analysis revealedthat the variant Ku80 protein was produced in similar amountsin both resistant (n = 4) and sensitive (n = 6) B-CLL samplesand in normal B lymphocytes (Figure 5F).

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Figure 5.. Constitutive increase in Ku70/80 heterodimer DNA-end binding activity. (A) Ku DNA-end binding activity in whole protein extracts from resistant (R) and sensitive B-CLL (S) cells (1 µg/lane) at the indicated times after treatment with 10 Gy ${gamma}$ -irradiation. The results shown are representative of those obtained in all extracts tested (n = 3 for resistant samples and n = 3 for sensitive samples). (B) Ku DNA-end binding activity (mean ± SEM in arbitrary units, AU) in 3 resistant B-CLL samples (R) and 3 sensitive B-CLL samples (S) at the indicated times after irradiation. (C) Untreated whole cell protein extracts (1 µg/lane) from the Ku80-deficient xrs6 cell line and the CHO-K1 line (expressing both Ku70 and Ku80 proteins). MO59J (DNA-PKcs deficient) and MO59K (normal levels of DNA-PKcs activity) were used as controls. (D) Untreated B-CLL lymphocyte protein extracts (5 µg, lane 1) were immunodepleted using 125 ng (lane 2) and 250 ng (lane 3) monoclonal Ku70 antibody, assayed for Ku DNA-end binding activity (1 µg protein extract/lane) (upper panel) and then subjected to Western blot (WB) analysis (lower panel). For supershift assays (lanes 4-5), samples were treated with 5 µg untreated B-CLL lymphocyte protein extract (lane 5) or with 250 ng polyclonal Ku70 antibody (lane 4), and then assayed for Ku DNA-end binding (1 µg of protein extract/lane). (E) Whole-cell extracts (5 µg) were obtained from representative sensitive and resistant B-CLL cell samples at the indicated times after irradiation. Extracts were subjected to electrophoresis on a 10% SDS polyacrylamide gel (DNA-PKcs analysis was carried out using a 6% SDS polyacrylamide gel). Proteins were then blotted onto polyvinylidenefluoride (PVDF) membranes and were detected using the appropriate antibodies. (F) Whole-cell extracts (5 µg) from 6 sensitive (S) and 4 resistant (R) untreated B-CLL cell samples, and 4 untreated normal B-cell samples from healthy donors (B cells) were subjected to Western blotting analysis as described in panel E. See Supplemental Figure S3 for more information.

   Discussion

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

The primary response of cells with excessive DNA damage is torepair the lesions. Maintenance of the switching mechanismsthat shift the cell from DNA repair to apoptosis is of centralimportance for avoiding progression to malignancy.
Previous investigations of the in vitro apoptotic response ofB cells from B-CLL patients to irradiation have revealed resistantand sensitive subsets.^20,21 Approximately 15% of B-CLL patientspresent B cells resistant to irradiation-induced apoptosis.We propose that human B-CLL cells can escape DNA damage-inducedapoptosis by up-regulating the NHEJ DNA repair system. In aprevious study, we showed that increased DNA damage repair wasassociated with the accumulation of an unusually high numberof chromosomal aberrations in the resistant cell subset.²² Irradiationhas been reported to induce apoptosis via DNA damage-independentprocesses such as generation of ceramide by the activated acidsphingomyelinase.⁴¹ We showed here that the sensitivity of the2 B-CLL cell subsets to irradiation-induced apoptosis was dependenton the response to DSBs. We found that B-CLL subsets that wereresistant or sensitive to irradiation-induced apoptosis werealso resistant or sensitive to apoptosis induced by NCS andthe topoisomerase II inhibitor VP-16. NHEJ is the predominantpathway for the repair of both NCS- and topoisomerase II-mediatedDNA damage: wild-type and repair-deficient yeasts and LIG4^-/-and Ku70^-/- cells, which are defective in NHEJ, are extremelysensitive to NCS^42,43 and to both VP-16 and ICRF-193.⁴⁴ We foundthat okadaic acid, an inhibitor of protein phosphatases 1 and2A, induced apoptosis in both resistant and sensitive B-CLLsamples, indicating the existence of a functional executivecell death pathway in resistant cells. Okadaic acid inducesapoptosis in many cell types including B-CLL cells.^39,45,46
Approximately 10% of B-CLL patients present p53 mutations andconsecutive drug resistance.⁴⁷ To test the possibility thatresistant B-CLL cells display p53 dysfunction and/or mutations,22 B-CLL samples (10 sensitive and 12 resistant samples) wereassessed for p53 status using a functional assay in yeasts⁴⁸and sequence-mutation analysis. Only 4 resistant B-CLL samplespresented both a nonfunctional p53 protein and a mutation inthe p53 gene (Blaise et al⁴⁹ and J.D., unpublished data, July2004). ATM is one of the signal transducers thought to be essentialfor the general DNA damage response.⁵⁰ The ATM gene is mutatedin 18% of B-CLL patients, and loss of heterozygosity (LOH) at11q22-23 is observed in 14% of cases.^51,52 P53 activity hasbeen reported to involve ATM.^53-55 However, none of the 10 B-CLLsamples displaying radio-resistant apoptosis and p53 wild type(p53wt) examined presented ATM LOH.⁴⁹ Thus, our data from previousstudies suggest that neither p53 nor ATM deficiencies can fullyexplain the resistance of some B-CLL cells to DNA damage-inducedapoptosis.
We previously found that DNA damage repair was enhanced in theresistant B-CLL subset, however, we also found that this rapidDNA repair was highly prone to errors.²² Considering that G₀yeast cells with unrepressed NHEJ capacity have an increasedfrequency of small-scale mutations, and thus large-scale chromosomalinstability,⁵⁶ and the fact that more than 95% of neoplasticB-CLL cells are in a G₀ quiescent state⁵⁷ (supplemental data,available on the Blood website; see the Supplemental Figureslink at the top of the online article), we sought whether thisDNA repair system could also define the cell susceptibilityto undergo or not DNA damage-initiated apoptosis. This hypothesisis also consistent with studies reported elsewhere in the literaturesuggesting that NHEJ plays a role in the control of the apoptoticresponse following DNA damage.^58,59 We found here that wortmannin,a known inhibitor of DNA-PKcs,²⁷ restored sensitivity to irradiation-inducedapoptosis to cells that were otherwise resistant to this celldeath pathway. Wortmannin enhances B-CLL cell cytotoxicity tochlorambucil by inhibiting DNA-PK activity.²⁶ Our results showedthat 1 µM wortmannin increased the incidence of apoptosisin irradiation-treated resistant B-CLL cells by 4- to 5-fold.However, at the concentrations used, wortmannin inhibits ATMand PI-3 K in addition to DNA-PKcs.²⁴ We also investigated theeffect of NU7026, a DNA-PKcs-specific inhibitor, at concentrationsof 10 µM on irradiation-induced apoptosis in the resistantcells. NU7026 enhances topoisomerase II inhibitor-induced cytotoxicity.²³Our results were consistent with this model: we found that 10µM NU7026 restored irradiation-induced apoptosis sensitivityto otherwise resistant cells as efficiently as wortmannin.
A striking finding of this study is that overall NHEJ and DNA-PKcsactivity increased 2- and 4-fold, respectively, in resistantB-CLL cells 15 minutes after exposure to irradiation. In contrast,only small increases of NHEJ and DNA-PKcs activity were detectedin the sensitive cells. We also found that both NU7026 and wortmanninsuppressed NHEJ and DNA-PKcs activity in the B-CLL extracts.These results show that the increases in DSB DNA repair andDNA-PKcs activity detected in resistant B-CLL cells after exposureto irradiation cannot be attributed to DNA-PK-independent repairor mechanisms involving other PI-3 kinases. We did not detectincreases in NHEJ activity in irradiation-treated EBV-transformedB cells. Although we did not investigate DNA-PK activity inthe normal B cells in detail, these results are consistent withthose obtained in our previous study showing that the sensitivityof the normal B cells to irradiation treatment was similar tothat of the sensitive B-CLL cell subset.²² Likewise, both NHEJand DNA-PK activity have been reported to be higher in samplesfrom patients with myeloid leukemias associated with concomitantDNA misrepair and in samples of B-CLL cells resistant to nitrogenmustard treatment than in normal B lymphocytes from healthydonors.^18,60 Interestingly, Ku80^-/- p53^-/- mice succumb to disseminatedpro-B-cell lymphoma before 3 months of age. Tumors result froma specific set of chromosomal translocations and gene amplificationsinvolving immunoglobulin heavy chain (IgH) and c-Myc, reminiscentof Burkitt lymphoma.⁶¹ DNA-PKcs-deficient mice also displayaccelerated aging and increased lymphoma.⁶² Moreover, mice withXRCC4 or ligase IV deficiencies die during late embryonic development.They also display extremely high levels of apoptosis in newlygenerated neurons throughout their developing nervous system.^63-65Although p53 deficiency allowed postnatal survival of XRCC4-deficientmice, they routinely succumbed to pro-B-cell lymphomas thathad chromosomal translocations, supporting a crucial role forthe NHEJ pathway as a caretaker of the mammalian genome.⁵⁸ Altogether,these results show that NHEJ deficiencies^58,61,62 or NHEJ up-regulation^22,60could potentially lead to genomic instability. Investigationof XRCC4 and ligase IV protein levels in B-CLL samples revealedthat the levels of these 2 proteins varied considerably betweenB-CLL cell samples, irrespective of their sensitivity to apoptosis.Our data suggest that the initial recognition of DSBs by theDNA-PK complex is the most crucial event for efficient NHEJDNA repair and escape of apoptosis.
We propose that constitutive high levels of DNA end-bindingby the Ku70/Ku80 heterodimer up-regulate DNA-PKcs and NHEJ activityand allow the resistant B-CLL subset to escape apoptosis despiteirradiation-induced DNA damage. We found that Ku70/Ku80 heterodimerDNA-binding activity was higher in the resistant B-CLL cellsthan in sensitive cells, both before and after irradiation treatment.These data support the idea that regulation of DNA-PK activityoccurs primarily through Ku.³ Other studies have reported thatDNA-PK activity in B-CLL cells is regulated by the Ku heterodimer.^18,66The authors proposed that DNA-PK activity is down-regulatedby a Ku80 variant.^17,40,66 However, we found that the productionof this variant form of Ku80 varied considerably between samplesfor both the resistant and sensitive B-CLL cells, as well asfor normal B lymphocytes. These results show that productionof the truncated Ku80 protein cannot explain the differencesin DNA-PKcs and NHEJ activity between the 2 B-CLL subsets. Studiesof the proteins interacting with Ku, the levels of Ku phosphorylation,and further biochemical studies will help us to determine howthe differences in Ku heterodimer DEB activity in the sensitiveand resistant B-CLL cell subsets lead to resistance to DNA damage-inducedapoptosis. Our findings demonstrate that overactive NHEJ DSBrepair allows human B-CLL cells to escape apoptosis in the presenceof irradiation-induced DNA damage. The deregulation of a potentiallymutagenic DNA repair system, such as NHEJ, may be one of thefirst steps toward carcinogenesis, as mutations in p53 and drugresistance occur as a consequence of DNA-damaging chemotherapyin B-CLL patients.⁴⁷

   Acknowledgements

We are grateful to the volunteer blood donors and to P. A. Jeggofor providing us with the pull-down DNA-PKcs protocol. We alsothank O. Delattre for the pSP65 substrate and T. Lindahl forthe DNA ligase IV antibody.

   Footnotes

Submitted July 28, 2004; accepted February 11, 2005.
Prepublished online as Blood First Edition Paper, February 17,2005; DOI 10.1182/blood-2004-07-2888.

Supported by grants from Association pour la Recherche sur leCancer, Ligue Nationale Contre Cancer, SociétéFrançaise du Cancer, Société Françaised'Hématologie, Commissariat à l'Energie Atomique,Fondation de France, Electricité de France, and Contractof European Community (CEC) RADINSTAB FIGH-1999-00003.

The online version of the article contains a data supplement.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Jozo Delic, Commissariat à l'Energie Atomique, Laboratoire de Radiobiologie et Oncologie, 18 route du panorama, B.P.6, 92265 Fontenayaux-roses, France; e-mail: jozo.delic{at}cea.fr.

   References

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Rich T, Allen RL, Wyllie AH. Defying death after DNA damage. Nature. 2000;407: 777-783.[CrossRef][Medline] [Order article via Infotrieve]

Richardson C, Jasin M. Frequent chromosomal translocations induced by DNA double-strand breaks. Nature. 2000;405: 697-700.[CrossRef][Medline] [Order article via Infotrieve]

Smith GC, Jackson SP. The DNA-dependent protein kinase. Genes Dev. 1999;13: 916-934.[Free Full Text]

Mimori T, Hardin JA. Mechanism of interaction between Ku protein and DNA. J Biol Chem. 1986;261: 10375-10379.[Abstract/Free Full Text]

Falzon M, Fewell JW, Kuff EL. EBP-80, a transcription factor closely resembling the human autoantigen Ku, recognizes single- to double-strand transitions in DNA. J Biol Chem. 1993;268: 10546-10552.[Abstract/Free Full Text]

Gottlieb TM, Jackson SP. The DNA-dependent protein kinase: requirement for DNA ends and association with Ku antigen. Cell. 1993;72: 131-142.[CrossRef][Medline] [Order article via Infotrieve]

Lees-Miller SP, Chen YR, Anderson CW. Human cells contain a DNA-activated protein kinase that phosphorylates simian virus 40 T antigen, mouse p53, and the human Ku autoantigen. Mol Cell Biol. 1990;10: 6472-6481.[Abstract/Free Full Text]

Calsou P, Delteil C, Frit P, Drouet J, Salles B. Coordinated assembly of Ku and p460 subunits of the DNA-dependent protein kinase on DNA ends is necessary for XRCC4-ligase IV recruitment. J Mol Biol. 2003;326: 93-103.[CrossRef][Medline] [Order article via Infotrieve]

Grawunder U, Wilm M, Wu X, et al. Activity of DNA ligase IV stimulated by complex formation with XRCC4 protein in mammalian cells. Nature. 1997;388: 492-495.[CrossRef][Medline] [Order article via Infotrieve]

Critchlow SE, Bowater RP, Jackson SP. Mammalian DNA double-strand break repair protein XRCC4 interacts with DNA ligase IV. Curr Biol. 1997;7: 588-598.[CrossRef][Medline] [Order article via Infotrieve]

Bernstein C, Bernstein H, Payne CM, Garewal H. DNA repair/pro-apoptotic dual-role proteins in five major DNA repair pathways: fail-safe protection against carcinogenesis. Mutat Res. 2002;511: 145-178.[CrossRef][Medline] [Order article via Infotrieve]

Shieh SY, Ikeda M, Taya Y, Prives C. DNA damage-induced phosphorylation of p53 alleviates inhibition by MDM2. Cell. 1997;91: 325-334.[CrossRef][Medline] [Order article via Infotrieve]

Woo RA, Jack MT, Xu Y, Burma S, Chen DJ, Lee PW. DNA damage-induced apoptosis requires the DNA-dependent protein kinase, and is mediated by the latent population of p53. Embo J. 2002;21: 3000-3008.[CrossRef][Medline] [Order article via Infotrieve]

Mayo LD, Turchi JJ, Berberich SJ. Mdm-2 phosphorylation by DNA-dependent protein kinase prevents interaction with p53. Cancer Res. 1997;57: 5013-5016.[Abstract/Free Full Text]

Jimenez GS, Bryntesson F, Torres-Arzayus MI, et al. DNA-dependent protein kinase is not required for the p53-dependent response to DNA damage. Nature. 1999;400: 81-83.[CrossRef][Medline] [Order article via Infotrieve]

Jhappan C, Yusufzai TM, Anderson S, Anver MR, Merlino G. The p53 response to DNA damage in vivo is independent of DNA-dependent protein kinase. Mol Cell Biol. 2000;20: 4075-4083.[Abstract/Free Full Text]

Muller C, Salles B. Regulation of DNA-dependent protein kinase activity in leukemic cells. Oncogene. 1997;15: 2343-2348.[CrossRef][Medline] [Order article via Infotrieve]

Muller C, Christodoulopoulos G, Salles B, Panasci L. DNA-dependent protein kinase activity correlates with c