Cell Proliferation and DNA Breaks Are Involved in Ultraviolet Light-induced Apoptosis in Nucleotide Excision Repair-deficient Chinese Hamster Cells

doi:10.1091/mbc.01-05-0225

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Originally published as MBC in Press, 10.1091/mbc.01-05-0225 on December 7, 2001

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Vol. 13, Issue 1, 348-361, January 2002

Cell Proliferation and DNA Breaks Are Involved in Ultraviolet Light-induced Apoptosis in Nucleotide Excision Repair-deficient Chinese Hamster Cells

Torsten R. Dunkern, and Bernd Kaina^*

Institute of Toxicology, Division of Applied Toxicology, University of Mainz, D-55131 Mainz, Germany

Submitted May 7, 2001; Revised October 10, 2001; Accepted October 22, 2001
Monitoring Editor: Mitsuhiro Yanagida

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

UV light targets both membrane receptors and nuclear DNA, thus evoking signals triggering apoptosis. Although receptor-mediatedapoptosis has been extensively investigated, the role of DNA damagein apoptosis is less clear. To analyze the importance of DNA damageinduced by UV-C light in apoptosis, we compared nucleotide excisionrepair (NER)-deficient Chinese hamster ovary cells (lines 27-1and 43-3B mutated for the repair genes ERCC3 and ERCC1, respectively)with the corresponding DNA repair-proficient fibroblasts (CHO-9and ERCC1 complemented 43-3B cells). NER-deficient cells werehypersensitive as to the induction of apoptosis, indicating thatapoptosis induced by UV-C light is due to unrepaired DNA basedamage. Unrepaired lesions, however, do not activate the apoptoticpathway directly because apoptosis upon UV-C irradiation requiresDNA replication and cell proliferation. It is also shown thatin NER-deficient cells unrepaired lesions are converted into DNAdouble-strand breaks (DSBs) and chromosomal aberrations by a replication-dependentprocess that precedes apoptosis. We therefore propose that DSBsarising from replication of DNA containing nonrepaired lesionsact as an ultimate trigger of UV-C-induced apoptosis. Inductionof apoptosis by UV-C light was related to decline in the expressionlevel of Bcl-2 and activation of caspases. Decline of Bcl-2 andsubsequent apoptosis might also be caused, at least in part, byUV-C-induced blockage of transcription, which was more pronouncedin NER-deficient than in wild-type cells. This is in line withexperiments with actinomycin D, which provoked Bcl-2 decline andapoptosis. UV-C-induced apoptosis due to nonrepaired DNA lesions,replication-dependent formation of DSBs, and activation of themitochondrial damage pathway is independent of functional p53for which the cells aremutated.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The main target of UV-C irradiation in living cells is nuclear DNA. The formation of DNA lesions such as pyrimidine dimersand TC(6-4) photoproducts inhibits DNA replication as well astranscription of RNA and causes chromosomal breakage, DNA recombination,mutations, and reproductive cell death (Friedberg et al., 1995).UV-C light also targets extranuclear macromolecules, inducingsignal transduction pathways via the activation of membrane receptorssuch as insulin receptor, platelet-derived growth factor, fibroblastgrowth factor, and epidermal growth factor receptor (Canman andKastan, 1996). Programmed cell death (apoptosis) induced by UV-Clight in various cell types has been proposed to be a consequenceof receptor activation (reviewed in Schwarz, 1998). This conclusionis based mainly on the finding that UV-C provokes clustering ofCD95R, which leads to activation of the apoptotic caspase network(Rehemtulla et al., 1997; Aragane et al., 1998). Another lineof evidence suggests activation of growth factor receptors tostimulate mitogen-activated protein kinase cascade, which activatestranscription factors targeting genes that are involved in cellsurvival and apoptosis (Canman and Kastan, 1996). However, themodel of receptor-mediated activation of apoptotic pathways incells exposed to a DNA-damaging agent does not clearly considernonrepaired DNA damage to be involved as a primary trigger ofapoptosis. It also does not allocate DNA repair to play a rolein defense againstapoptosis.

A major defense mechanism against the deleterious effects of UV-C light is nucleotide excision repair (NER). NER-deficientcells are generally hypersensitive to the cytotoxic, mutagenic,and genotoxic effects of UV-C light (Wood and Burki, 1982; Westerveldet al., 1984; Stefanini et al., 1986; Weber et al., 1988; Weedaet al., 1990; reviewed in Friedberg et al., 1995). The hypersensitivityof repair-deficient cells to the cell-killing effect as measuredby reproductive cell death (colony formation) could theoreticallybe due to apoptosis, necrosis, mitotic death, or irreversiblecell cycle arrest (Orren et al., 1997). The contribution of nonrepairedDNA damage induced by various genotoxins to either one of theseendpoints, notably apoptosis, still needs to be clarified. Also,it is not clear whether DNA damage-induced pathways interact,by cooperation or inhibition, with receptor-mediatedsignaling.

UV-C light activates the p53 tumor suppressor protein. This activation has been shown to control cell cycle arrest, blockingG1/S and G2/M transition (Agarwal et al., 1995; Guillouf et al.,1995). This is supposed to permit cells to repair DNA damage beforepassing through S phase or entering mitosis (Ponten et al., 1995;Poon et al., 1996). Furthermore, p53 has been shown to be directlyinvolved in DNA repair (Ford and Hanawalt, 1997; Smith et al.,2000; Zhou et al., 2001) and in the regulation of the expressionof DNA repair genes such as alkyltransferase (Rafferty et al.,1996; Grombacher et al., 1998). These functions of p53 are obviouslyprotective, reducing genotoxicity of DNA-damaging agents. In contrast,p53 is a major player of apoptotic signaling (Reinke and Lozano,1997), being involved in down-regulation of antiapoptotic Bcl-2(Haldar et al., 1994; Miyashita et al., 1994) and up-regulationof proapoptotic Bax (Miyashita and Reed, 1995) and CD95R/FasR(Muller et al., 1998). It has been suggested that stalling ofthe transcription machinery by UV-C light-induced DNA lesionsleads to activation of p53, thus initiating apoptosis (Ljungmanet al., 1996, 1999). p53 induction by UV light has also been shownto occur in human epidermal cells where it causes apoptosis andsunburn (Brash et al., 1996). Apoptosis, however, can also beinduced in a p53-independent manner upon exposure of cells toUV-C light and other kinds of DNA-damaging agents (Strasser etal., 1994), which was recently shown to be true also for p53-deficientmouse fibroblasts (Lackinger and Kaina, 2000). This indicatesthe existence of hitherto unknown p53-independent mechanisms involvedin DNA damage-triggeredapoptosis.

UV-C light blocks DNA replication, as all genotoxic agents do (Painter and Howard, 1982). Immediate replication blockage isdue to inhibition of replication initiation and, at high-doselevel, to DNA chain elongation (Kaufmann and Cleaver, 1981; Drissiand Lee, 1998; McGregor, 1999). UV-C induces DNA breaks and homologousas well as nonhomologous DNA recombination, which are detectablein the first post-treatment mitosis as chromatid-type aberrations.This process is strictly bound on replication of DNA containingnonrepaired lesions. It has been suggested that blockage of DNAreplication is causally related to the formation of DNA double-strandbreaks (DSBs) and chromosomal aberrations because of nucleaseattack at stalled replication forks (Kaina, 1985, 1998). DSBsare also formed as a consequence of replication of DNA containingother kinds of damage, such as the alkylation lesion O⁶-methylguanine. This lesion has previously been shown to be majorlyresponsible for cell killing in alkyltransferase-deficient cells(reviewed in Kaina et al., 1997b) and to be ultimately involvedin activating the apoptotic pathway (Tominaga et al., 1997; Kainaet al., 1997b; Meikrantz et al., 1998; Hickman and Samson, 1999;Ochs and Kaina, 2000). It has also been proposed that DSBs arethe ultimate trigger of O⁶-methylguanine-induced apoptosis (Ochs and Kaina, 2000). In viewof these findings, the question arises as to a possible involvementof DSBs in UV-C light-induced apoptosis. Herein, we show thatapoptosis induced by UV-C light in fibroblasts requires cell cycleprogression and DNA replication and is related to DNA strand breakformation, which causes Bcl-2 decline and caspase activation ina p53-independentmanner.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Materials

All antibodies used for Western blotting were purchased from Santa Cruz Biotechnology (Santa Cruz, CA). We used the antibodiesanti-Bcl-2 (clone C-2), anti-Fas (clone M-20), and anti-ERK2 (C-14).The p53-promoter-mdm2-luciferase plasmid was provided by Dr. M.Oren (Rehovot, Israel). The general cell-permeable caspase inhibitorN-benzyloxycarbonyl-Val-Ala-Asp-fluoromethylketone (zVAD-FMK)was purchased from R & D Systems (Minneapolis, MN). Fluoresceinisothiocyanate (FITC)-coupled zVAD-FMK is a product of Promega(Madison, WI). FITC-coupled anti-bromo-deoxyuridine (BrdU)-antibodyis a product of BD Biosciences (San Jose,CA).

Cell Lines

In our experiments, we used the parental Chinese hamster ovary cell line CHO-9 and the UV-C-hypersensitive derivatives 43-3Band 27-1 (Wood and Burki, 1982). 43-3B cells are mutated in theERCC1 gene (Westerveld et al., 1984), whereas 27-1 cells are mutatedin the ERCC3 gene (Weeda et al., 1990). The corresponding geneproducts, ERCC1 (5' endonuclease) and ERCC3 (helicase), are requiredfor the incision step of the NER pathway. Therefore, cells inwhich these genes are inactivated are unable to perform NER. Stablycomplemented 43-3B cells by transfection with the cloned gene(herein designated as 43-3B/ERCC1 cells) were kindly providedby Dr. R. Wood (Pittsburgh, PA). Cells were cultured in DMEM/F-12medium containing Glutamax (Invitrogen, Carlsbad, CA) and 5% fetalcalf serum at 37°C in an atmosphere containing 7% CO₂. Establishedmouse fibroblasts (the line BK4 generated in this laboratory)and primary mouse fibroblasts (Lackinger and Kaina, 2000) werecultured in DMEM containing 10% fetal calf serum. Transfectedcell lines were selected by G418 (1.5 mg/ml).

UV-C Treatment

Before UV-C treatment, the culture medium was removed, cells were irradiated, and the medium was added again immediately afterirradiation. The UV-C lamp used was calibratedroutinely.

Survival Experiments

Four hundred cells were seeded into 6-cm dishes. Then 8-10 h later, the culture medium was removed and cells were irradiatedwith different doses of UV-C. One week later colonies were fixedwith methanol and stained with 1.25% Giemsa, 0.125% crystal violetfor counting. Survival was expressed in relation to the untreatedcontrol. Values are given as the mean of three independentexperiments.

Determination and Quantification of Apoptosis

For quantification of apoptotic and necrotic cells, flow cytometric analyses with annexin V-FITC and propidium iodide-stainedcells were performed. Treated and untreated cells were trypsinized,washed in ice-cold phosphate-buffered saline (PBS), and resuspendedin 30 µl of cold annexin V binding buffer (10 mM HEPES pH 7.4,0.14 M NaCl, 0.25 mM CaCl₂ · 2H₂O, 0.1% bovine serum albumin,wt/vol). After addition of 1.5 µl of annexin-V-FITC (BD PharMingen,San Diego, CA) cells were incubated for 15-30 min in the dark.At least 264 µl of binding buffer and 6 µl of propidium iodide(50 µg/ml) were added per sample. Samples were analyzed on a FACSortflow cytometer (BD Biosciences). For each sample, 10,000 cellswere analyzed. The number of apoptotic and necrotic cells wascalculated using a computer program (Cell Quest software; BD Biosciences).For semiquantitative determination of apoptosis, DNA ladderingassays were performed as described (Ioannou and Chen, 1996). DNAof UV-C treated or untreated cells was isolated 48 h afterirradiation.

Equal amounts of DNA of each sample were separated on a 1.5% agarose gel. To evaluate the number of cells with enhanced apoptoticcaspase activity, treated and untreated cells were incubated inthe dark in medium containing 10 µM FITC-VAD-FMK. Thereafter,cells were trypsinized and analyzed by flow cytometry. For simultaneousdetermination of DNA content and caspase activity, cells weretrypsinized after incubation with FITC-VAD-FMK, washed with ice-coldPBS, and fixed in ice-cold 70% ethanol for a minimum of 1 h. Thereafter,cells were centrifuged, resuspended in 300 µl of PBS, and treatedwith RNase A for 30 min at room temperature. Finally, propidiumiodide was added to a final concentration of 16 µg/ml and 10,000cells were analyzed by flowcytometry.

BrdU-Enzyme-linked Immunosorbent Assay (ELISA)

For determination of DNA synthesis we used the Cell Proliferation ELISA BrdU assay (Roche Molecular Biochemicals, Mannheim,Germany) according to the manufacturer's protocol. Briefly, cellscultured in 96-microwell plates were pulse labeled for 1 h with10 µM BrdU. Thereafter, cells were fixed and DNA was denaturatedfor 30 min. After 1 h of incubation with a peroxidase-coupledanti-BrdU-antibody, cells were washed three times with PBS. Thereafter,peroxidase substrate (tetramethylbenzidine) was added for 30 minand measurements were performed on an ELISA reader (405nm).

Neutral Single Cell Gel Electrophoreses (SCGE)

Treated and untreated cells were trypsinized and washed with PBS. Cell concentration was equilibrated to 1 × 10⁶/ml. Cell suspension (10 µl) was resuspended in 120 µl of 0.5%low melting point agarose at 37°C, spotted onto a microscope slide,and covered with a coverslip. After keeping on ice for 5 min andremoving the coverslip, slides were incubated in neutral lysisbuffer (2.5 M NaCl, 100 mM EDTA, 10 mM Tris, 1% Na-laurylsarcosinate,pH 7.5) for 1 h. Thereafter, slides were placed into an electrophoreseschamber filled with electrophoreses buffer (90 mM Tris, 90 mMboric acid, 2 mM EDTA, pH 7.5). Thereafter, electrophoreses wereperformed, slides were washed in water, fixed in ethanol, andair dried. Analysis of 50 cells/sample was performed automaticallyafter staining with 20 µg/ml ethidium bromide on a fluorescencemicroscope by using a charge-coupled device camera connected toa personal computer and analysis software (Fuji Imaging, Tokyo,Japan).

Chromosomal Preparations

Treated and untreated cells were incubated in medium in the presence of 50 ng/ml colcemid for 2 h. Thereafter, cells weretrypsinized. Trypsinized cells were collected together with themedium, centrifuged, washed with PBS, and centrifuged again. Thereafter,the cell pellet was resuspended and incubated in 75 mM KCl for7 min at room temperature and centrifuged. Afterward, the cellpellet was resuspended in 2 ml of 75 mM KCl, and 12 ml of ice-coldmethanol/acetic acid (3:1) was added. After centrifugation, cellswere resuspended in methanol/acetic acid and incubated at $-$ 20°Cfor a minimum of 30 min. Thereafter, cells were again centrifugedand resuspended in methanol/acetic acid. The cell pellet was resuspendedin 1 ml of methanol/acetic acid (1:1), spotted onto an ice-coldwet microscope slide, and fixed by heating. After Giemsa staining,the preparations were analyzed under a microscope. At least 100metaphases were scored per measurepoint.

BrdU-In Situ Staining

Immediately after irradiation of cells grown on a coverslip, BrdU was added into the culture medium up to a final concentrationof 10 µM/ml. After a postincubation period of 36 h, cells werewashed with cold PBS, fixed onto the coverslip, and DNA was denaturatedfor 30 min. Thereafter, cells were incubated with an FITC-coupledanti-BrdU antibody in the dark for 30 min. Then cells were washedthree times for 5 min with PBS. For chromatin staining, cellswere incubated for 5 min in a 10-µl solution (1 µg/ml). The percentageof BrdU-stained cells with apoptotic chromatin morphology wasdetermined using a fluorescencemicroscope.

Transfection Experiments

Cells were stably transfected with Bcl-2 expression plasmid (Dimmeler et al. 1999) as previously described (Ochs and Kaina,2000).

Reporter Gene Assay

Cells were transfected with a p53-driven mdm-2-promoter-luciferase plasmid by means of the calcium phosphate coprecipitationmethod as described above. Transfected cells were split into twoculture dishes serving as a control and treatment dish, respectively.Ten hours thereafter cells were either treated with 15 J/m² UV-C or left untreated. Twelve hours after treatment cells weretrypsinized, washed in cold PBS, and resuspended in 0.25 M TrispH 8.0. Thereafter, cells were frozen in liquid nitrogen and thawedquickly at 37°C for three times. Finally, the suspension was centrifugedfor 10 min at 10,000 × g and protein concentration of the supernatantwas determined. Protein (10 µg) of each probe in a total volumeof 20 µl was used for luciferase activity measurement. Measurementswere made using the Berthold luminometerSirius.

Preparation of Cell Extracts

Trypsinized treated and untreated cells were washed with cold PBS, resuspended in sonification buffer (20 mM Tris-HCl pH 8.5,1 mM EDTA, 5% glycerin, 1 mM dithiothreitol, 0.5 mM phenylmethylsulfonylfluoride), and sonified. The resulting suspension was centrifugedwith 20,000 × g for 15 min. Supernatants were collected and proteinconcentration wasdetermined.

Western Blot Analysis

Protein (20-30 µg) of the probes was separated on a 7.5-12% SDS polyacrylamide gel. Thereafter, proteins were blotted ontoa nitrocellulose transfer membrane (Protran; Schleicher & Schuell,Dassel, Germany) for 3 h or, in some experiments, overnight. Membraneswere blocked for 2 h in 5% (wt/vol) milk powder in PBS containing0.1% Tween 20 (PBT), incubated for 2 h with the primary antibody(1:3000-5000 dilution), washed three times with PBT, and incubatedfor 1 h with a horseradish peroxidase-coupled secondary antibody1:3000 (Amersham Biosciences AB, Uppsala, Sweden). After finalwashing with PBT (3 times for 10 min each) blots were developedby using a chemiluminescence detection system (Amersham BiosciencesAB).

Transcription Measurement

Treated and untreated cells were pulse labeled for 1 h with 0.5 µCi/ml [³H]uridine triphosphate. After trypsinization, cells were suckedonto glass microfiber filters, washed carefully with 10% trichloroaceticacid and three times with aqua dest., and finally with ethanol.Thereafter, filters were air dried and measured by scintillationcounting.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

NER-deficient Cells Are Hypersensitive to UV-C-induced Apoptosis

The NER-deficient CHO cell lines 27-1 and 43-3B mutated in ERCC3 and ERCC1 gene, respectively, are known to be hypersensitiveto UV-C light. The killing response of these cells in comparisonwith the wild-type and ERCC1-complemented 43-3B cells as determinedby reduction in colony formation is shown in Figure 1A. Annexinstaining and flow cytometric measurement showed that these cellsare also hypersensitive to the induction of apoptosis. Withinthe dose range in which survival of complemented and wild-typecells was not yet affected 27-1 and 43-3B cells showed a dose-dependentincrease in apoptosis (Figure 1B). The frequency of necrosis (forquantification, see MATERIALS AND METHODS) was only slightly enhancedin the DNA repair-deficient cells (our unpublished data ).

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Figure 1. Cell-killing response and apoptosis in NER-deficient cells treated with UV-C light. (A) Survival of CHO-9, 43-3B/ERCC1, 27-1, and 43-3B cells as a function of UV-C dose, as determined by colony formation assay. (B) Frequency of apoptosis of CHO-9, 43-3B/ERCC1, 43-3B, and 27-1 cells as a function of dose of UV-C (measured 48 h after irradiation). (C) Apoptotic DNA laddering pattern in 27-1 cells (left) as a function of time after UV-C treatment (10 J/m²). Flow cytometric quantification of 27-1 cells with enhanced caspase activity 24 and 48 h after UV-C irradiation (10 J/m²) as determined by FITC-zVAD-FMK staining (right).

To confirm increase of the induction of apoptosis by UV-C light in the NER-deficient cells and to determine the time of initiationof apoptosis after UV-C treatment, DNA laddering assays were performed.As demonstrated in Figure 1C, apoptotic DNA degradation started~15 h after UV-C irradiation in the NER-deficient cells. We alsomeasured overall caspase activation by flow cytometry of FITC-VAD-FMK-stainedcells. Induction of caspases was first observed 15 h after UV-Ctreatment and further increased with the time of postincubation(Figure 1C,right).

UV-C-induced Apoptosis in NER-deficient Cells Requires Cell Cycle Progression

To address the question of whether cell cycle progression is necessary for UV-C-induced apoptosis, we comparatively investigatedUV-C-induced apoptosis in serum-starved and nonstarved cells.Serum starvation of CHO-9 and 27-1 cells for 3 days strongly reducedcell proliferation (Figure 2A) as well as DNA synthesis (Figure2B). Flow cytometric cell cycle analysis revealed accumulationof starved cells in G1 (>88% G1 fraction; our unpublished data).Starvation of CHO-9 and 27-1 cells followed by UV-C irradiationresulted in a significant reduction (by ~50%) of apoptosis comparedwith proliferating cells (Figure 2C). In this experiment, we usedan equitoxic dose (in terms of colony formation) of UV-C for irradiationof CHO-9 and 27-1 cells (40 and 10 J/m², respectively), which yielded nearly identical rates of apoptosisin both cell types. Because with an equitoxic dose of UV lightthe same frequency of proliferating cells underwent apoptosis(Figure 2C), it is reasonable to conclude that apoptosis is amain cause of UV-C-induced cytotoxicity, both in NER-deficient27-1 and wild-type cells. We should note that the frequency ofnecrosis was not significantly enhanced in 27-1 cells. Overall,the data obtained with the NER-deficient mutant clearly indicatethat DNA damage is the main trigger of UV-C-induced apoptosis.The data also show that UV-C-induced apoptosis requires cell proliferation.

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Figure 2. UV-C-induced apoptosis in serum-starved cells. (A) Growth curves of CHO-9 and 27-1 cells cultured with or without fetal calf serum. (B) DNA synthesis of CHO cells cultured for 72 h with (+) or without ( $-$ ) serum as determined by BrdU-ELISA. (C) Frequency of apoptosis in CHO-9 and 27-1 cells irradiated with 40 and 10 J/m², respectively, as measured by annexin staining. Cells were cultured for 72 h with or without serum before irradiation and apoptosis was measured 48 h after irradiation.

One could argue that serum starvation may alter the sensitivity of cells to UV-C light due to growth factor depletion. Toreject this argument, we analyzed UV-C-induced apoptosis withoutchanging the serum concentration as a function of cell density,which determines the confluence status of the adherent growingcells. As shown in Figure 3A, the DNA replication rate declinedwith increasing cell density. If cells seeded at different densitywere treated with UV-C light, the frequency of apoptosis inducedin CHO-9, 27-1, and 43-3B cells was inversely related to celldensity (Figure 3B). Obviously, the cells became more refractoryto UV-C-induced apoptosis when they were not allowed to replicateextensively.

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Figure 3. Dependency of UV-C-induced apoptosis on proliferation. (A) DNA synthesis as a function of the number of cells seeded. (B) Frequency of apoptosis 48 h after UV-C irradiation (10 J/m² for 27-1 and 43-3B cells; 40 J/m² for CHO-9 cells) as a function of cell seeding number. (C) Flow cytometric quantification of UV-C (40 J/m²)-induced apoptotic sub-G1 cells in exponentially growing and confluent primary mouse fibroblasts as measured 48 h after irradiation.

To gain further support for the conclusion of proliferation dependence of the induction of apoptosis by UV-C light, we comparedconfluent and subconfluent primary mouse fibroblasts. These cellsexhibit contact inhibition more severely than CHO cells. As shownin Figure 3C, contact-inhibited mouse fibroblasts displayed avery strong suppression of UV-C-induced apoptosis if they weretreated in a confluent state. The effect was clearly more pronouncedthan in the CHO cell lines (38 vs. 55% reduction, respectively),which is likely due to nearly complete growth inhibition of mousemonolayerscultures.

UV-C Light Induces Proliferation-dependent DSBs in NER-deficient Cells

Previously, we proposed that DNA DSBs and/or chromosomal aberrations arising from them act as a distal trigger of genotoxin-inducedapoptosis (Ochs and Kaina, 2000; Lips and Kaina, 2001). To seewhether this could also be true for NER-deficient cells irradiatedwith UV-C, we analyzed both endpoints comparatively in CHO-9 andNER-deficient 27-1 cells as a function of dose and time. The dataare shown in Figure 4A. Chromosomal aberrations were significantlyinduced by low doses of UV-C light in NER-deficient cells, whereasonly a slight induction was observed within this dose range (0-10J/m²) in CHO-9 and 43-3B/ERCC1 cells. Chromosomal aberrations wereobserved as early as 14 h after irradiation and increased in frequencywith increasing postincubation time.

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Figure 4. UV-C-induced DNA breakage is proliferation dependent. (A) Frequency of UV-C-induced chromosomal aberrations in 43-3B, 27-1, 43-3B/ERCC1, and CHO-9 cells as a function of UV-C dose (left; 22 h post-treatment) and time (right; 8 J/m² of UV-C). (B) UV-C-induced DSBs as a function of time. Cells were irradiated with a UV-C dose of 10 J/m² and analyzed by means of neutral SCGE. (C) DSBs as a function of UV-C dose 20 h post-treatment, as determined by neutral SCGE. (D) UV-C light-induced DSBs as measured 20 h after UV-C irradiation in 27-1, 43-3B, 43-3B/ERCC1 (ERCC1), and CHO-9 cells, which were determined by neutral SCGE assay. (E) UV-C-induced DSBs 20 h after UV-C treatment (10 J/m²) in 27-1 cells cultivated in medium not containing ( $-$ ) or containing (+) fetal calf serum, as determined by neutral SCGE.

To see whether NER-deficient cells are vulnerable to DSB formation, the frequency of DSBs was analyzed by means of neutralSCGE. DSB induction was observed already 8 h after UV-C irradiationin NER-deficient cells (Figure 4B). The induction was a functionof dose; it increased notably in NER-deficient 27-1 cells withdoses between 5 and 30 J/m² (as measured 20 h after irradiation; Figure 4C). Increase ofDSB frequency was also observed in 43-3B cells irradiated with10 J/m² (Figure 4D). In NER-proficient cells a similar frequency of DSBswas observed with 40 J/m² (Figure 4D). To see whether the formation of DSBs by UV-C lightdepends on DNA synthesis and cell cycle progression, we comparedserum-starved and nonstarved cells treated with UV-C light. Thefrequency of DSBs was clearly reduced in irradiated starved cells(Figure 4E).

One could argue that DNA strand breaks observed by SCGE are merely a reflection of apoptotic internucleosomal DNA cleavage.Therefore, we compared the induction of DSBs in cells treatedwith UV-C alone and UV-C plus zVAD-FMK, which is a general caspaseinhibitor. Post-treatment of UV-C-irradiated cells with zVAD-FMKreduced apoptosis frequency nearly to the level of untreated cells(Figure 5A). However, application of zVAD-FMK did not affect thelevel of UV-C-induced DSBs as determined by SCGE (Figure 5B).This indicates that DSBs measured by neutral SCGE were not resultingfrom apoptotic internucleosomal DNA fragmentation.

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Figure 5. Reduction of apoptosis but not DSBs after UV-C irradiation by zVAD-FMK. (A) Frequency of apoptosis in UV-C-irradiated (10 J/m²) 27-1 cells treated or not treated with the general caspase inhibitor zVAD-FMK (100 µM). Cells were analyzed 48 h after UV-C treatment by annexin staining and flow cytometry. (B) UV-C (10 J/m²) induced DSBs in 27-1 cells treated or not with the general caspase inhibitor zVAD-FMK (100 µM). Cells were harvested 20 h after irradiation and subjected to neutral SCGE.

Most UV-C-induced Apoptotic Cells Underwent S Phase after Irradiation

As revealed by time course experiments, DNA breaks and aberrations preceded the appearance of apoptotic cells. To elucidatewhether apoptotic cells have passed through S phase after UV-Cirradiation, we labeled UV-C-irradiated cells deficient in NERwith BrdU immediately after irradiation and analyzed DNA synthesisand apoptosis (by means of apoptotic nuclear morphology) in thesame individual cells by using anti-BrdU antibody as well as 4,6-diamidino-2-phenylindole(DAPI) staining in situ. As shown in Table 1, ~70% of the apoptoticcells were clearly positive for BrdU staining, which is characteristicfor replicating cells. This indicates that most cells have progressedthrough S phase before they were triggered to die by apoptosis.

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Table 1. Percentage of cells undergoing apoptosis after DNA replication Quantification was performed by simultaneous staining for DNA synthesis and apoptotic nuclear morphology after UV-C irradiation (36 h post-treatment; 10 J/m²) of 27-1 cells. BrdU-labelling had been performed for 36 h after UV-C irradiation.

NER-deficient cells pass after UV-C irradiation through the cell cycle (otherwise chromosomal aberrations would not be detectablein the first post-treatment mitoses), but do not significantlyproliferate later on (our unpublished data). Therefore, UV-C-inducedapoptosis due to DNA damage is likely to be initiated in the postexposurecell cycle, after the cells have passed through mitosis. By simultaneousflow cytometric determination of DNA content and overall caspaseactivity in treated and untreated cells, we demonstrate that apoptoticcaspase activation occurs in all cell cycle phases of UV-C $---$ irradiatedcells. Most caspase activity was detectable, however, in the apoptoticsub-G1 population and in cells out of G1 phase (Figure 6A). Becausemost of the apoptotic cells underwent S phase after irradiation(Table 1), it is reasonable to conclude that G1 phase cells exhibitingstrongly enhanced caspase activity undergo apoptosis after thefirst post-treatment division, i.e., in the first postexposurecell cycle.

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Figure 6. Cell cycle-specific activation of caspases and p53 activity in UV-C-irradiated 27-1 cells. (A) Flow cytometric dual color staining for DNA content (PI) and caspase activity of untreated (top, left) and UV-C-treated (10 J/m²; top, right) 27-1 cells. The bottom panels show quantitative cell cycle distributions 36 h after treatment. (B) Determination of p53-regulated mdm2 promoter activity after transient transfection of the construct followed by UV-C irradiation (15 J/m²). Cells were harvested 12 h after treatment of BalbC, CHO-9, and 27-1 cells and analyzed for luciferase activity. (C) Expression of CD95R after UV-C treatment (10 J/m²) of 27-1 cells and of doxorubicin-treated (0.5 µg/ml) CHO-9 and BK4 cells, as shown by Western blot analysis.

UV-C-induced Apoptosis in NER-deficient Cells Does not Require Functional p53 and Fas Receptor (Fas-R) Up-Regulation

Because p53 is considered to be a key regulator of apoptosis upon DNA damage, we analyzed whether CHO-9 and 27-1 cells possessp53 transactivation activity. We used mdm2-promoter-luciferaseconstruct, which is clearly inducible in p53-expressing BalbCcells upon UV-C irradiation. In CHO-9 and 27-1 cells, however,there was no induction of the p53-driven promoter (Figure 6B),supporting the view that p53 is mutated and therefore functionallyinactive in CHO-9 cells. Obviously, p53 is not involved in UV-C-inducedapoptosis in this cell type. We also measured the expression levelof Fas-R (CD95R). As shown in Figure 6C, treatment of cells withUV-C did not provoke up-regulation of Fas-R. In a control experimentwith doxorubicin, which was reported to induce Fas-R (Fulda etal., 2000), we also did not find induction, whereas in mouse fibroblasts(BK4 cells expressing p53 wild type) Fas-R was up-regulated (Figure6C). These data indicate that CHO-9 cells and the correspondingNER-defective derivatives are unable to respond with Fas up-regulationto UV-C irradiation. Similar data were obtained with Fas ligand,which proved also not to be induced in CHO-9 cells upon UV-C treatment(our unpublisheddata).

Decline of Bcl-2 in NER-deficient Cells

To see whether Bcl-2 level is related to UV-C-induced apoptosis, Bcl-2 was quantified as a function of time after UV-C exposure.As shown in Figure 7A, Bcl-2 decreased in the repair competentcells 10-20 h after irradiation and thereafter recovered, returningto control level (Figure 7A, left). In NER-deficient cells, however,a dramatic decrease of Bcl-2 was observed and recovery to thecontrol level did not occur (Figure 7A, right). As revealed bythe time course experiments, in both NER-deficient cell typesdecrease in Bcl-2 preceded the induction of apoptosis (Figure7A, right). One could argue that NER-competent cells would respondin the same way as repair-deficient cells, albeit at higher doselevel at which UV-C-induced DNA lesions cannot be repaired intime. This is indeed the case. As shown in Figure 7B, Bcl-2 declinedin CHO-9 cells irradiated with 40 J/m² to the same extent as in 27-1 cells irradiated with 10 J/m². With this low dose, CHO-9 and ERCC-1-complemented 43-3B cellsdid not display significant Bcl-2 decline. Because NER-deficientcells showed decline of Bcl-2 at a lower UV-C dose level thanrepair-competent cells, the data indicate that Bcl-2 becomes down-regulatedin response to nonrepaired UV-C-induced DNA damage.

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Figure 7. Decline of Bcl-2 in NER-deficient cells after UV-C irradiation. (A) Relative Bcl-2 amount (continuous line) and apoptosis frequency (dotted line) as a function of time after UV-C irradiation (10 J/m²) of CHO-9 and 43-3B/ERCC1 cells (left) and NER-deficient 27-1 and 43-3B cells (right). (B) Expression of Bcl-2 in CHO-9 and 27-1 cells treated with 40 and 10 J/m², respectively (left), as well as expression of Bcl-2 in 10 J/m² UV-C-treated CHO-9 and 43-3B/ERCC1 cells, as shown by Western blot analysis. (C) Transcriptional activity as a function of UV-C dose in CHO-9 and 27-1 cells 4 h after treatment. (D) Transcriptional activity as a function of concentration of actinomycin D in CHO-9 and 27-1 cells, as determined 4 h after treatment. (E) Frequency of apoptosis in 27-1 cells as a function of concentration of actinomycin D. (F) Expression of Bcl-2 in 43-3B and 27-1 cells after actinomycin D treatment, as shown by Western blot analysis. The ERK2 signal illustrates equal protein loading on the gel.

Trancription Blockage in NER-deficient Cells and Apoptosis

To elucidate the effect of UV-C irradiation on transcription, RNA synthesis was measured by uridine incorporation. Transcriptionwas blocked significantly in the dose range of 2-20 J/m² with 27-1 cells eliciting a clearly stronger response than thewild type (Figure 7C). This finding raised the question of whetherincreased transcription blockage due to nonrepaired DNA damageis related to Bcl-2 decline and the induction of apoptosis inNER-defective cells. If true one would suppose that inhibitionof transcription by a treatment other than UV-C would cause thesame effect. To prove this, we treated cells with the transcriptioninhibitor actinomycin D (Act D). The agent caused a clear suppressionof transcription (Figure 7D) and, within the same concentrationrange, induction of apoptosis (Figure 7E). We next analyzed theeffect of the RNA synthesis inhibitor on Bcl-2 expression, usinga concentration of Act D that induced the same yield of apoptosisas 10 J/m² of UV-C light (the Bcl-2 expression studies described above wereperformed by treating cells with 10 J/m² UV-C). As shown in Figure 7F, Act D caused decrease in Bcl-2with a time course similar to that observed after UV-C treatmentof 27-1 and 43-3B cells. This supports the view that transcriptionblockage after exposure to UV-C light is involved in Bcl-2 declineand the induction of apoptosis in NER-deficient cells. To furtherprove the involvement of Bcl-2 in apoptosis, Bcl-2 was stablyoverexpressed by transfection in 27-1 cells (unpublished expressiondata), which were subjected for apoptosis measurements. Figure8 shows the average response of Bcl-2 transfectants in comparisonwith 27-1 and vector-transfected 27-1 cells. Bcl-2 transfectantswere significantly protected against the induction of apoptosisupon UV-C irradiation. They were not protected as to the levelof UV-C-induced necrosis.

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Figure 8. Effect of Bcl-2 overexpression in 27-1 cells on UV-C-induced apoptosis. 27-1 cells were transfected with a myc-bcl-2 construct and seven Bcl-2-overexpressing clones were established. Clones, vector transfected cells, and untransfected cells were irradiated (10 J/m² UV-C) and flow cytometric annexin measurements were performed 48 h later (***, highly significant difference with p < 0.05). Ordinate: average yield (%) of apoptotic and necrotic cells.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Although it is known that UV-C light induces apoptosis in various cell types (reviewed in Schwarz, 1998), the mechanism stillneeds to be elucidated. UV-C light acts upon nuclear as well ascytoplasmic targets such as CD95/Fas (Rehemtulla et al., 1997;Aragane et al., 1998). Although several lines of evidence suggestthat DNA damage and activation of the CD95/Fas receptor contributeindependently to apoptosis (Schwarz, 1998), it is not known howimportant the DNA damage and the receptor triggered pathway fora given cell type are and how UV-C-induced DNA damage triggersthe response. In this investigation, we demonstrate that hypersensitivityto UV-C light of NER mutants, which are deficient in the removalof UV-C-induced DNA damage (Weber et al., 1988; Hayashi et al.,1998), is due to massive induction of apoptosis (as determinedby annexin staining, electrophoretic DNA laddering, and activationof caspases) but not to a significant extent to necrosis. Theincreased apoptotic response of NER-deficient cells indicatesthat nonrepaired UV-C-induced DNA damage acts as a primary triggerof apoptosis. The data confirm a recent report demonstrating repairof pyrimidine dimers by photolyase in mammalian cells to protectagainst apoptosis (Chigancas et al., 2000). One might argue thatthe apoptotic pathway is evoked specifically in repair-deficientcells. This however is not true. Treatment of DNA repair-proficientCHO-9 and ERCC1-complemented 43-3B cells with an equitoxic dose(as measured by loss of colony-forming ability) of UV-C resultedin a level of apoptosis comparable with that observed in the repair-deficientmutants. This indicates that reproductive cell death induced byUV-C light in normal repair-proficient CHO fibroblasts is alsocaused by apoptosis triggered by nonrepaired DNAdamage.

The major cell-killing lesions induced by UV-C light are pyrimidine dimers and (6-4) photoproducts (Friedberg et al., 1995).If nonrepaired UV-C-induced DNA lesions trigger apoptosis, thequestion arises as to whether the primary DNA damage itself (i.e.,the base damage) constitutes the signal activating the apoptoticpathway or whether other (secondary) lesions arising from themare involved. The primary base damage is very likely not sufficientin triggering apoptosis, at least in fibroblasts, because apoptosisis a rather late response that requires cell proliferation (asdiscussed below). A critical candidate of secondary lesions couldbe DSBs, which have previously been shown to be very efficientin inducing apoptosis (Lips and Kaina, 2001). UV-C light doesnot induce DSBs per se. However, DSBs can be formed during DNAreplication due to nuclease attack at stalled replication forks,which has been proposed to be a critical event not only for UV-Cbut also for other genotoxic agents (Kaina et al., 1997a; Kaina,1998). To examine whether unrepaired UV-C light-induced DNA lesionsare converted into DSBs by means of DNA replication, we analyzedthe induction of DSBs by neutral SCGE. We also analyzed chromosomalaberrations arising from them. It is shown that UV-C induces significantlymore DSBs and chromosomal aberrations in NER-deficient cells comparedwith NER-proficient fibroblasts. This indicates that primary nonrepairedUV-C light-induced DNA lesions are indeed converted into DSBs.The induction of DSBs was dependent on DNA replication becauseconfluent G1 phase-arrested and serum-starved cells suppressedin DNA replication exhibited a reduced rate of UV-C-induced DSBs.This supports the hypothesis that DSBs induced by UV-C light aregenerated in S phase during the replication of DNA, which containslesions blockingreplication.

It is of much interest that not only the frequency of DSBs but also the frequency of apoptosis was significantly reduced inUV-C light-treated cells that were nonreplicating due to serumstarvation. This supports the hypothesis that DSBs are criticallyinvolved in UV-C light-induced apoptosis. Because serum starvationmay cause side effects, we verified the finding by using cellsof different confluence and proliferation status. These experimentsrevealed that UV-C-induced apoptosis is indeed a function of proliferation,because apoptosis in CHO cells was reduced with increasing confluenceand reduced DNA replication capacity (as measured by BrdU incorporation)of the cell population. As demonstrated by simultaneous BrdU labelingand nuclear staining of apoptotic cells, at least 70% of apoptoticcells have passed through S phase upon UV-C treatment. Replicationdependence of UV-C light-induced apoptosis was confirmed withprimary mouse fibroblasts exhibiting strong contact inhibition.These cells become highly refractory to UV-C-induced apoptosiswhen they were kept in a confluent state upon irradiation. Overall,the data indicate that the induction of apoptosis by UV-C lightrequires DNAreplication.

Apoptosis could be initiated in the postreplicative G2 phase or in the cell cycle thereafter. Because most UV-C-exposed cellsundergo mitosis (in which chromosomal damage becomes visible)it is pertinent to conclude that apoptosis is initiated in thefirst postexposure cell cycle. This is supported by the fact thatsignificant activation of caspases occurred in cells out of G1phase 36 h after irradiation. Because the first postexposure mitoticcells exhibit massive chromosomal aberrations, it is temptingto speculate that loss of genetic material due to chromosomaldeletions and translocations leading to a disturbed balance ofgene expression could be critically involved in the initiationof apoptosis. Chromosomal aberrations as a trigger of apoptosishave been proposed before for another cellular system (Kaina etal., 1997a) and gain support by recent data from other investigations(De Santis et al., 2001).

To study in more detail the molecular mechanism of apoptosis due to UV-C-induced DNA damage, we proved the involvement ofvarious pro- and anti-apoptotic proteins. One major player isp53, which is inducible by UV-C light leading either to cell cyclearrest or apoptosis, depending on the cellular system (Agarwalet al., 1995; Guillouf et al., 1995; Liebermann et al., 1995;Pellegata et al., 1996). CHO cells, however, do not express detectablep53 protein (our unpublished data). Also, luciferase assays witha p53-regulated mdm2-promoter construct showed lack of transactivatingactivity of p53 in UV-C-treated CHO cells (in contrast to p53-expressingmouse fibroblasts serving as a control). This demonstrates thatp53 is functionally inactive in CHO-9 cells and the correspondingmutants we were working with. Inactivation of p53 in CHO cellshas also been reported by another group (Lee et al., 1997). Itindicates that p53 does not play a role in the induction of apoptosisin our cellular system. This is important to note because it hasbeen shown that UV-C activates the CD95 receptor, which is p53regulated (Muller et al., 1998). Furthermore, p53 has been shownto regulate the expression of proapoptotic Bax (Miyashita andReed, 1995). We should note that we did not observe up-regulationof the CD95R and CD95L as well as Bax after UV-C irradiation inCHO cells undergoing apoptosis (this article; and our unpublisheddata).

There is increasing evidence that DNA damage-induced apoptosis is regulated via the mitochondrial apoptotic pathway, withBcl-2 the most prominent protein involved. Bcl-2 is mainly localizedin the outer mitochondrial membrane forming heterodimers withproapoptotic Bax, thus preventing homodimerization of Bax (reviewedin Antonsson and Martinou, 2000). Homodimerized Bax generatespores in the mitochondrial membrane, resulting in release of cytochromec, apoptosis-inducing factor, and subsequent caspase-9 activation(Narita et al., 1998). Based on this model, down-regulation ofBcl-2 leads to induction of apoptosis, whereas up-regulation canprevent it. We show here that Bcl-2 is indeed down-regulated afterUV-C irradiation in 27-1 and 43-3 cells. We also overexpressedBcl-2 by transfection with an expression vector in NER-deficient27-1 cells, thus protecting them from UV-C-induced apoptosis.In NER-proficient cells the decline in Bcl-2 level occurred onlyslightly and transiently and was observed only upon treatmentwith high doses of UV-C light. This is in contrast to NER-deficient27-1 and 43-3B cells where Bcl-2 was not detectable anymore ~72h after irradiation. Bcl-2 decline was first observed ~8 h afterUV-C treatment and nearly paralleled the generation of DSBs. Ittherefore clearly preceded the induction of apoptosis. The resultsare in line with the view that Bcl-2 decline is a consequenceof DSB formation upon UV-C treatment. The finding that ionizingirradiation as well as electroporation of PvuII, which both efficientlyinduce DSBs and apoptosis, are also able to induce down-regulationof Bcl-2 in p53-deficient cells (Lips and Kaina, 2001) supportsthishypothesis.

It is well known that UV-C-induced DNA lesions block transcription, which has been suggested to act as a trigger of apoptosis(Ljungman and Zhang, 1996; Ljungman et al., 1999). To prove theinvolvement of transcription blockage in apoptosis in NER-deficientfibroblasts, we compared transcriptional activity of UV-C-treated27-1 cells with the corresponding wild type. We observed a dramaticreduction of transcription in NER-deficient cells but not to thesame extent in the wild type upon UV-C irradiation, which is obviouslydue to unrepaired DNA lesions. Therefore, transcription blockagemust also be considered to be involved in the induction of apoptosis.This conclusion gains support from experiments reported hereinin which transcription was inhibited by actinomycin D, which,at the same time, induced apoptosis. Actinomycin D also causeddown-regulation of Bcl-2, indicating that transcriptional inhibitioncould be a second component activating the Bcl-2-dependent apoptoticpathway. We should note that we were unable to block UV-C-inducedapoptosis completely in growth-arrested CHO cells. The residualamount of apoptotic cells observed after growth inhibition couldthus be due to transcription blockage, which is not influencedby the state of proliferation of thecells.

The time sequence of events, as measured in NER-deficient cells, is summarized in Figure 9. It becomes obvious that the inductionof DSBs and aberrations coincide with the Bcl-2 decline, whichclearly precedes the appearance of apoptotic cells. The resultstherefore support a model suggesting that unrepaired UV-C-inducedDNA lesions are converted into DSBs and aberrations by replication,leading to down-regulation of Bcl-2 and finally caspase activation.This model provides at the same time a simple explanation forthe finding that UV-C-induced apoptosis in fibroblasts is, atleast in part, replication dependent. Transcriptional inhibitionmay also come into play as a second (minor) component, causingactivation of the mitochondrial apoptotic pathway upon the inductionof DNA damage by UV-C light. This process appears to be independentof p53. It would be interesting to see whether the mechanism proposedis generally operating in fibroblasts and other cell types, notablyp53-mutated tumor cells, and whether it competes with receptor-triggeredapoptotic pathways.

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Figure 9. Time course of effects induced by UV-C light in NER-deficient cells. Apoptosis, DSBs, chromosomal aberrations (percentage of aberrant cells) as well as Bcl-2 expression are shown at various time points after irradiation (10 J/m²) of 27-1 cells. Values are calculated as percentage relative to the maximum value.

	ACKNOWLEDGMENTS

We gratefully acknowledge Dr. R. Wood for providing stably complemented 43-3B/ERRC1 cells, Dr. M. Oren for a gift of the mdm2-promotorreporter plasmid, and Dr. S. Dimmeler for Bcl-2 expression plasmid.This work was supported by the Deutsche Forschungsgemeinschaft(SFB 519/B4 and Ka 724/8-4), by Stiftung Rheinland Pfalz for Innovation,and by a Ph.D. grant of the University of Mainz (to T.D.).

	FOOTNOTES

^* Corresponding author. E-mail address: kaina{at}mail.uni-mainz.de.

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.01-05-0225. Article and publication date are at www.molbiolcell.org/cgi/doi/10.1091/mbc.01-05-0225.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Cancer Res., June 1, 2008; 68(11): 4347 - 4351.
[Abstract] [Full Text] [PDF]

D. G. Soares, A. E. Escargueil, V. Poindessous, A. Sarasin, A. de Gramont, D. Bonatto, J. A. P. Henriques, and A. K. Larsen
From the Cover: Replication and homologous recombination repair regulate DNA double-strand break formation by the antitumor alkylator ecteinascidin 743
PNAS, August 7, 2007; 104(32): 13062 - 13067.
[Abstract] [Full Text] [PDF]

E. Despras, P. Pfeiffer, B. Salles, P. Calsou, S. Kuhfittig-Kulle, J. F. Angulo, and D. S.F. Biard
Long-term XPC Silencing Reduces DNA Double-Strand Break Repair
Cancer Res., March 15, 2007; 67(6): 2526 - 2534.
[Abstract] [Full Text] [PDF]

P. G. Smiraldo, A. M. Gruver, J. C. Osborn, and D. L. Pittman
Extensive Chromosomal Instability in Rad51d-Deficient Mouse Cells
Cancer Res., March 15, 2005; 65(6): 2089 - 2096.
[Abstract] [Full Text] [PDF]

P.-K. Lo, S.-Z. Huang, H.-C. Chen, and F.-F. Wang
The Prosurvival Activity of p53 Protects Cells from UV-Induced Apoptosis by Inhibiting c-Jun NH2-terminal Kinase Activity and Mitochondrial Death Signaling
Cancer Res., December 1, 2004; 64(23): 8736 - 8745.
[Abstract] [Full Text] [PDF]

Y. Mi, S. D. Thomas, X. Xu, L. K. Casson, D. M. Miller, and P. J. Bates
Apoptosis in Leukemia Cells Is Accompanied by Alterations in the Levels and Localization of Nucleolin
J. Biol. Chem., February 28, 2003; 278(10): 8572 - 8579.
[Abstract] [Full Text] [PDF]

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				P. C.H. Li, E. Lam, W. P. Roos, M. Z. Zdzienicka, B. Kaina, and T. Efferth Artesunate Derived from Traditional Chinese Medicine Induces DNA Damage and Repair Cancer Res., June 1, 2008; 68(11): 4347 - 4351. [Abstract] [Full Text] [PDF]

				D. G. Soares, A. E. Escargueil, V. Poindessous, A. Sarasin, A. de Gramont, D. Bonatto, J. A. P. Henriques, and A. K. Larsen From the Cover: Replication and homologous recombination repair regulate DNA double-strand break formation by the antitumor alkylator ecteinascidin 743 PNAS, August 7, 2007; 104(32): 13062 - 13067. [Abstract] [Full Text] [PDF]

				E. Despras, P. Pfeiffer, B. Salles, P. Calsou, S. Kuhfittig-Kulle, J. F. Angulo, and D. S.F. Biard Long-term XPC Silencing Reduces DNA Double-Strand Break Repair Cancer Res., March 15, 2007; 67(6): 2526 - 2534. [Abstract] [Full Text] [PDF]

				P. G. Smiraldo, A. M. Gruver, J. C. Osborn, and D. L. Pittman Extensive Chromosomal Instability in Rad51d-Deficient Mouse Cells Cancer Res., March 15, 2005; 65(6): 2089 - 2096. [Abstract] [Full Text] [PDF]

				P.-K. Lo, S.-Z. Huang, H.-C. Chen, and F.-F. Wang The Prosurvival Activity of p53 Protects Cells from UV-Induced Apoptosis by Inhibiting c-Jun NH2-terminal Kinase Activity and Mitochondrial Death Signaling Cancer Res., December 1, 2004; 64(23): 8736 - 8745. [Abstract] [Full Text] [PDF]

				Y. Mi, S. D. Thomas, X. Xu, L. K. Casson, D. M. Miller, and P. J. Bates Apoptosis in Leukemia Cells Is Accompanied by Alterations in the Levels and Localization of Nucleolin J. Biol. Chem., February 28, 2003; 278(10): 8572 - 8579. [Abstract] [Full Text] [PDF]