Institute of Pharmacy and
1 Institute of Toxicology, University of Mainz, D-55099 Mainz, Germany and
2 Imperial Cancer Research Fund, Clare Hall Laboratories, South Mimms, Hertfordshire EN6 3LD, UK
3 To whom correspondence should be addressedEmail: epe{at}mail.uni-mainz.de
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Abstract |
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Abbreviations: Fpg protein; formamidopyrimidine-DNA glycosylase; 8-oxoG; 7,8-dihydro-8-oxoguanine; Ro19-8022, [R]-1-[(10-Chloro-4-oxo-3-phenyl-4H-benzo[a]quinolizin-1-yl)-carbonyl]-2-pyrrolidinemethanol; ROS; reactive oxygen species.
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Introduction |
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The generation of oxidative DNA damage is counteracted in all species by specific repair mechanisms (57). One of the key repair enzymes in eukaryotic cells is Ogg1 protein, a DNA glycosylase that removes 7,8-dihydro-8-oxoguanine (8-oxoG) and other oxidative guanine modifications from the nuclear and mitochondrial DNA (8,9). Ogg1 is a functional, but not structural, analogue of the bacterial Fpg protein. Ogg1 deficiency in yeast, as well as Fpg deficiency in bacteria, results in a spontaneous mutator phenotype (10,11). GCTA transversions, which are the characteristic type of mutation caused by 8-oxoG due to its ability to pair with adenine, are increased specifically. Recently, 23-fold elevated spontaneous mutation rates were also detected in the liver of homozygous ogg1/ null mice (12,13) and all additional mutations appeared to be GC
TA transversions. The background level of 8-oxoG in the chromosomal DNA of untreated animals, which probably reflects the balance between the continuous generation and removal of this modification (steady-state level), was significantly higher in the liver of ogg1/ mice than in that of wild-type animals. Moreover, the level of 8-oxoG in the mutant mouse liver at 14 weeks of age was nearly 2-fold higher than at 9 weeks of age, which suggests an accumulation rate of 12 000 modifications per diploid cell per week (13).
To further characterize the consequences of an Ogg1 deficiency, we have analysed the steady-state levels of oxidative base modifications sensitive to Fpg protein in various organs and along the lifespan of ogg1 knockout mice. The results indicate that the accumulation of oxidative DNA modifications is tissue-specific, i.e. it is much more pronounced in hepatocytes than in several other cell types, most probably due to the high oxygen metabolism in the liver. An age-dependent increase of oxidative damage in ogg1/ mice indicates that either oxidative stress increases with age or the relevant cellular defence mechanisms become less efficient.
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Materials and methods |
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[R]-1-[(10-Chloro-4-oxo-3-phenyl-4H-benzo[a]quinolizin-1-yl)-carbonyl]-2-pyrrolidinemethanol (Ro19-8022) was a gift from Hoffmann-LaRoche AG (Basel, Switzerland).
Preparation of hepatocytes, splenocytes and kidney and testis cells from ogg1/and wild-type mice
Hepatocytes from ogg1/ and control mice were isolated by a modified two-step collagenase perfusion technique as previously described (15). Briefly, mice were anaesthetized with an intraperitoneal injection of pentobarbital (60 mg/kg), the liver was perfused in situ via the vena portae for 15 min with an EGTA-containing buffer at 37°C. The perfusion was continued with a collagenase buffer for 30 min. All buffers were carbogen-equilibrated before and during preparation, the flow did not exceed ~10 ml/min. After perfusion, the liver was removed and the hepatocytes carefully dissociated in suspension buffer, the suspension filtered through gauze (100 µm pore size). Cells were pelleted by centrifugation (10 min at 50 g) and resuspended in fresh suspension buffer (15) three times. The viability of the hepatocytes was determined by trypan blue (4 g/l) exclusion and ranged between 30 and 80%. The hepatocytes were subjected to analysis by alkaline elution (see below) within 1 h.
For the isolation of splenocytes, the spleen was cut into small pieces with surgical scissors in 10 ml trypsin/EDTA buffer (0.5 g/l trypsin, 0.2 g/l EDTA, 140 mM NaCl, 3 mM KCl, 8 mM NaH2PO4, 1.5 mM KH2PO4, pH 7.4) and incubated for 10 min at 37°C with gentle shaking. The reaction was stopped by the addition of 40 ml suspension buffer. Cells were pelleted by centrifugation (10 min at 150 g) and resuspended in an erythrocyte lysis buffer (155 mM NH4Cl, 10 mM KHCO3, 1 mM EDTA, pH 7.4) for 5 min on ice. Thereafter, the cells were pelleted again and resuspended in fresh suspension buffer. The viability of the splenocytes as determined by trypan blue exclusion ranged between 65 and 85%.
Kidney cells were prepared in a similar way, except that the treatment with trypsin/EDTA was replaced by an incubation in collagenase buffer for 90 min at 37°C. Cells could be cryopreserved in suspension buffer containing 10% DMSO using a slow freezing protocol (15) and stored in liquid nitrogen.
Testes and seminal ducts of male mice (aged 20.526.5 months) were cut into pieces and gently shaken in pre-chilled suspension buffer for 10 min. The suspension was pelleted by centrifugation at 50 g for 10 min and left at room temperature to allow vital spermatocytes to swim into the supernatant. After 30 min, the supernatant (containing the spermatocytes) was removed from the pellet and the cells were counted in a Neubauer chamber. The percentage of motile spermatocytes in the supernatant was 8090%.
Quantification of Fpg-sensitive modifications in DNA by the alkaline elution technique
The alkaline elution protocol followed the method of Kohn et al. (16) with modifications (17,18). The number of cells applied to each filter was 5x105 in the case of the hepatocytes and 1x106 in all other cases to compensate for the higher DNA content (polyploidy) of the hepatocytes. The sum of modifications sensitive to Fpg protein and single-strand breaks was determined following incubation of the cellular DNA for 60 min at 37°C with 1 µg/ml Fpg protein immediately after cell lysis. Under these conditions, the incision by the enzyme at sensitive DNA modifications has been shown to be completed (18). The numbers of modifications incised by Fpg protein were obtained by subtraction of the number of single-strand breaks observed in experiments without the enzyme. Elution curves obtained with -irradiated cells were used for calibration, assuming that 6 Gy generate 1 single-strand break per 106 bp (16). When induced modifications (rather than background levels) were to be quantified (repair assays), the slopes observed with untreated control cells (steady-state levels) were subtracted.
Determination of repair rates in cultured fibroblasts
To induce additional oxidative base damage for the determination of repair rates, spontaneously immortalized fibroblasts (106 cells/ml) were exposed to the photosensitizer Ro19-8022 (0.05 µM) in the presence of visible light from a 1000 W halogen lamp (Philips PF811) at a distance of 38 cm in Ca2+ and Mg2+-free PBS (140 mM NaCl, 3 mM KCl, 8 mM Na2HPO4, 1 mM KH2PO4, pH 7.4) at 0°C for 10 min, corresponding to 14 kJ/m2 between 400 and 500 nm. Treatment results in the induction of 0.5 Fpg-sensitive base modifications per 106 bp (~60% of which were identified as 8-oxoG) and relatively few other DNA modifications and does not reduce the viability of the cells (19). To remove the damaging agents, the treated cells were washed twice with Ca2+ and Mg2+-free PBS. Subsequently, the cells were resuspended in complete medium, incubated for various times under culture conditions at 37°C and analysed for unrepaired DNA modifications, as described above.
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Results |
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The results (Figure 1) indicate that the steady-state level of Fpg-sensitive modifications in the hepatocytes of ogg1/ mice was 2.8-fold higher than in wild-type mice. In contrast, no significant difference was observed for the other tissues.
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In order to analyse the influence of cell proliferation, we (i) determined the steady-state levels of Fpg-sensitive base modifications in proliferating and confluent immortalized embryonic fibroblasts derived from ogg1/ mice and (ii) compared the repair rates of additionally induced Fpg-sensitive base modifications in confluent and replicating ogg1/ fibroblasts.
There was no significant increase of the steady-state level of Fpg-sensitive DNA modifications when cultured ogg1/ fibroblasts reached confluence and were kept confluent for 8 days (data not shown). Therefore, the balance between the generation and removal of the oxidative base modifications is not instantly affected by DNA replication.
The repair kinetics in confluent and proliferating fibroblasts of additional Fpg-sensitive base modifications induced by exposure to the photosensitizer Ro19-8022 in the presence of light (19) is shown in Figure 4. Both for the ogg1/ and wild-type fibroblasts, similar repair rates were observed in dividing and non-dividing cells. Therefore, the previously described significant repair of Fpg-sensitive modifications in ogg1/ cells (12), which is ~4-fold slower than in wild-type cells, does not depend on cell proliferation. A putative replication-coupled repair mechanism for 8-oxoG can be ruled out.
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Discussion |
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The results further indicate that the tissue-specific accumulation of oxidative DNA damage in liver compared with other tissues cannot be explained by the lower level of cell turnover since (i) cell-cycle arrest alone does not change the level of oxidative DNA damage and (ii) the residual repair rate in ogg1/ fibroblasts is the same in proliferating and confluent cells (Figure 4). Therefore, it appears likely that a higher rate of generation of oxidative DNA damage rather than a reduced rate constant of removal is responsible for the selective accumulation in liver. The residual (back-up) repair activity in ogg1/ cells (Figure 4
) probably is sufficient to keep the steady-state levels at a minimum in most tissues, at least in the absence of additional oxidative stress, but it is too low to prevent an increase of the steady-state level in the case of metabolically highly active cells such as hepatocytes.
The residual repair activity in ogg1/ cells (t1/2 16 h) suggests that a balance between endogenous generation and removal of oxidative modifications (steady-state) is reached within days. Therefore, the age-dependent increase of the steady-state levels in the hepatocytes of ogg1/ mice (Figure 2
) is an indication that either the cellular antioxidant defence system deteriorates with age or the endogenous oxidative stress increases gradually. Experimental support for both effects has been described and forms the basis of free radical theories of ageing (2,23,24).
The absence of a significant age-dependent accumulation of oxidative DNA damage in hepatocytes of wild-type mice (Figure 2) contrasts with a previously observed 23-fold increase of 8-oxoG in the liver of wild-type rats during their lifespan (25). An experimental difference that could explain the discordant findings is that the technique described here excludes the possibly highly oxidized DNA from disintegrated or apoptotic cells and from mitochondria.
The nature of the back-up repair system remains to be established. The recently observed OGG1-independent transcription-coupled repair of 8-oxoG (26) cannot fully explain that >50% of all Fpg-sensitive modifications induced in ogg1/ cells are repaired (Figure 4), even if it is assumed that the photosensitizer might damage transcribed regions of the genomic DNA more efficiently than non-transcribed DNA. A hypothetically related replication-coupled repair mechanism is excluded by the repair in confluent cells. Nucleotide excision repair cannot be ruled out, although the comparison of spontaneous mutation frequencies in yeast ogg1 and rad14 single and double mutants provided only partial support for such an assumption (27).
The back-up repair and the resulting absence of a significant accumulation of oxidative DNA damage in most tissues could explain why the incidence of cancer and other age-related diseases proposed to be associated with oxidative DNA damage is not clearly increased in ogg1/ mice. In the case of the liver, the low level of cell proliferation might prevent cancer development in the absence of a tumor promoting activity. This notion is supported by recent data indicating that a significant age-dependent accumulation of spontaneous point mutations (including GCTA transversions) only takes place in proliferating tissue (28). However, the consequences of an OGG1 defect may become apparent in combination with other mutations that affect either the generation or the removal of oxidative DNA damage. Indeed, mutations in the OGG1 gene have been observed in some human tumors of the kidney, lung and other organs (29,30) and also in a mouse strain characterized by accelerated senescence (31). This would support the notion that OGG1 is a `caretaker' gene whichwhen mutatedunder some conditions can facilitate tumor development by increasing spontaneous mutation rates (32). The analysis of double knockout mice and cells will allow further studies of the relevance of oxidative DNA damage and its repair.
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Acknowledgments |
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References |
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