Abstract
Cultured primary human cells inevitably enter a state of replicative senescence for which the specific molecular trigger is unknown. We show that the single-strand telomeric overhang, a key component of telomere structure, is eroded at senescence. Expression of telomerase prevents overhang loss, suggesting that this enzyme prevents senescence by maintaining proper telomere structure. In contrast, progressive overhang loss occurs in cells that avoid senescence through the inactivation of p53 and Rb, indicating that overhang erosion is the result of continuous cell division and not a consequence of senescence. We thus provide evidence for a specific molecular alteration in telomere structure at senescence and suggest that this change, rather than overall telomere length, serves to trigger this state.
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Two main hypotheses have been proposed to explain the mechanism governing the replicative lifespan of primary human cells1,2,3,4. The first suggests that cultured cells suffer from physiologic stress and cumulative damage that ultimately trigger senescence. The second postulates that an intrinsic counting mechanism triggers senescence after a predetermined number of cell generations. The 'telomere length' hypothesis is based on the latter model and argues that the progressive telomere shortening that occurs during successive divisions induces senescence once telomeres erode to a critical length3,5. Consistent with this hypothesis, expression of telomerase, which halts telomere erosion, prevents senescence6,7.
Some important experimental findings are not easily explained by the telomere length hypothesis. In most senescent cells, telomeres are still quite long, often averaging 5–10 kilobases (kb)5,8. There are many examples of cells that carry much shorter telomeres yet retain the ability to divide9,10,11. Thus, short telomeres per se are not incompatible with continued cellular division. Moreover, experimental acceleration of telomere shortening does not affect the onset of senescence12.
We speculated that another aspect of telomere structure, distinct from overall length, might govern the onset of senescence. Telomeric DNA consists of a double-strand region composed of TTAGGG repeats, which terminates in a 3′ single-strand G-rich overhang (refs. 13–16; Fig. 1a). The telomeric overhang has been implicated as a critical component of telomere structure that is required for proper telomere function17,18,19. We therefore undertook to examine whether changes in the overhang occur during senescence.
To assess the length of the telomeric overhang, we used a recently developed method termed telomere–oligonucleotide ligation assay (T-OLA; ref. 20). In this assay, radiolabeled oligonucleotides complementary to the telomeric overhang are annealed to genomic DNA, ligated and then electrophoretically separated (Fig. 1a). The length of the ligation products and their radioactive intensity then provide an indication of the length of the overhangs present in the sample.
We carried out a series of control experiments to assess the accuracy and sensitivity of T-OLA. First, we denatured a known number of double-strand DNA molecules composed of 200 and 350 base pairs (bp) of tandem telomeric repeats and mixed these with yeast genomic DNA (serving as a surrogate for non-telomeric genomic DNA). T-OLA analysis of this reconstructed system yielded products with maximal lengths of 168 and 312 nucleotides (nt), respectively (Fig. 1b), indicating that the assay is sensitive enough to detect telomeres present in total genomic DNA and provides a reasonably accurate representation of overhang length. In the absence of template denaturation, we detected only a faint signal, and a template with a randomly chosen sequence produced no signal (Fig. 1b).
We next treated genomic DNA samples from human BJ foreskin fibroblasts with various enzymes predicted to affect overhang length. We found that treatment with each of the enzymes affected T-OLA product length in the expected manner (Fig. 1c; see also ref. 20). Importantly, treatment with Bal31, a single-strand specific endonuclease, or with ExoI, a single-strand specific exonuclease, resulted in loss of most T-OLA signal (Fig. 1c). An oligonucleotide carrying a mismatched telomeric sequence did not yield a T-OLA signal, and an oligonucleotide complementary to the C-rich strand produced only a faint signal (Fig. 1d). Finally, T-OLA signal intensities showed a near-linear response to increases in input genomic DNA (Fig. 1e). These experiments show that T-OLA detects the presence of 3′ single-strand telomeric overhangs with high specificity and sensitivity.
We used T-OLA to examine the telomeric overhang in BJ fibroblasts grown in culture from an early passage until they reached senescence. By population doubling (PD) 80, the proliferation rate of these cells is greatly reduced, and by PD 100 virtually all cells become senescent, exhibiting a typical flat morphology and senescence-associated β-galactosidase activity (Fig. 2h). T-OLA done on DNA from early-passage BJ cells (PD 25) generated a ladder of products reaching a maximal detected length of 624 nt (Fig. 2a). Previous reports have estimated that the overhang ranges from 50 to 400 nt in various cell types including BJ fibroblasts13,14,15,16,20. Although most overhangs may be in this size range, T-OLA is probably sensitive enough to detect longer overhangs if they are present in the sample.
As BJ cells were passaged, T-OLA products remained constant in intensity and maximal length up to PD 68 (Fig. 2a). Notably, senescent BJ cells at PD 106 had markedly lower signal intensity, with products reaching a maximal detected length of only 384 nt (Fig. 2a). Densitometric analysis indicated that the total signal intensity of T-OLA products in senescent cells dropped to 19% of that observed in young cells (Fig. 2e). Thus, both the maximal length and total signal intensity were lower in senescing BJ cells, indicating substantially shorter overhangs in these cells. We also examined the telomeric overhangs in BJ cells by an alternative method, non-denaturing telomeric restriction fragment (TRF) Southern blotting15. Similar to our results with T-OLA, we found that the telomeric overhang in senescent (PD 106) BJ cells was considerably shorter than that of younger cells (Fig. 2b).
We also carried out T-OLA analysis on an additional normal human cell line, MRC5 human lung fibroblasts. These cells enter senescence between PD 49 and PD 59. T-OLA analysis indicated that senescing MRC5 cells had much shorter telomeric overhangs (Fig. 2c,f), and this was also shown by non-denaturing TRF Southern-blot analysis (data not shown).
We observed that in both BJ and MRC5 cells, the T-OLA products of 120 nt and longer were markedly less abundant in senescent cells, whereas products of 48–96 nt remained nearly constant in intensity throughout the lifespan of the cells (Fig. 2a,c). Densitometric analysis indicated that in the senescent cells 65% of the signal intensity was observed in products <120 nt, as compared with 37% in early passage cells. It has been shown that telomeres can exist in a 'T-loop' structure18. The formation of the T-loop depends on the presence of the telomeric overhang, which invades upstream double-strand telomeric DNA, and it has been suggested that at least 100 nt of overhang participate in the formation of this structure18,21. Our data suggest that during senescence most overhangs drop below 100 nt, potentially disrupting the T-loop or another telomeric structure.
The kinetics of overhang loss differ from those of overall telomere shortening. Telomere shortening has been shown to occur at a constant rate of approximately 50–100 bp per division in various cell types5,16,22. We observed this type of overall telomere shortening in both BJ (Fig. 2b) and MRC5 cells (Fig. 2d,g). In contrast, we found that telomeric overhang lengths remained constant during early passages and then dropped abruptly at senescence (Fig. 2e,f). This difference in kinetics indicates that overhang length is not a direct reflection of overall telomere length.
Ectopic expression of the catalytic subunit of telomerase (TERT) prevents senescence in many cell types6,7. Because telomerase adds telomeric repeats to the 3′ end of the telomere, it could directly extend the telomeric overhang23. We found that BJ and MRC5 cells overexpressing TERT carried telomeric overhangs similar in length to those present in early-passage cells, or, in some cases, longer (Fig. 2a–c,e,f). Thus, sequences added to the 3′ telomeric end by telomerase extend overall telomere length but also generate longer single-strand overhangs. We suggest that the means by which telomerase prevents entry to senescence is by maintaining telomeric overhang and, therefore, proper telomere structure, rather than by extending double-strand repeats.
It is possible that loss of the telomeric overhang is a consequence of the senescence program itself and, as such, does not have a causal role in inducing this state. To test this, we examined whether the telomeric overhang was lost in cells that bypass senescence after inactivation of the senescence effector proteins p53 and Rb, which is achieved by overexpression of the SV40 large T-antigen. Such cells continue to divide beyond the senescence point until they reach a second proliferative barrier termed crisis24. At crisis, the bulk of the double-strand telomeric DNA is lost, resulting in genomic catastrophe and massive cell death. BJ and MRC5 cells expressing large T-antigen were passaged beyond the point where they normally enter senescence and into crisis. Notably, the telomeric overhangs in these cells were progressively lost during propagation to an extent similar to that observed in senescent cells (Fig. 3a,b). Thus, overhang loss seems to be a direct result of continued cellular division and not of the senescence program itself. Furthermore, the continued growth of cells lacking normal telomeric overhangs indicates that inactivation of the p53 and Rb pathways renders cells refractory to signals induced by telomeric overhang loss. The fraction of such cells in the population is thus allowed to progressively increase, explaining the progressive mode of overhang erosion that is observed by T-OLA in these cells. In a normal cell population, however, cells losing their overhangs will senesce and be eliminated from the population. Therefore, substantial overhang loss is observed only when most of the cells in the population senesce.
To test whether the quiescent state of senescent cells contributes to overhang loss, we induced growth arrest in BJ fibro-blasts by contact inhibition. T-OLA signal intensity in arrested cells was 80% of that in proliferating cells (Fig. 4a). When cells were held under these quiescent conditions for 4 weeks, we observed a slight further decrease in signal to 68% of that observed in proliferating cells (Fig. 4a). We conclude that the state of quiescence can contribute to a minor loss of telomeric overhang but cannot explain the substantial loss (to 19%) observed in senescence (Fig 2e).
To determine whether overhang loss is a general cellular response to physiologic stress, we exposed BJ cells to DNA damage–inducing agents, to oxidative stress conditions or to metabolic stresses. Some treatments caused a considerable reduction in T-OLA signal, specifically methyl-nitro-nitroso-guanidine, hydrogen peroxide and cycloheximide (Fig. 4b,c). The former two have been suggested to specifically damage G-rich telomeric DNA25. None of the treatments reduced T-OLA signal to the same magnitude of the reduction observed in senescent BJ cells, indicating that loss of the telomeric overhang is not a general cellular response to physiologic stress. Instead, we suggest that certain physiologic stresses suffered by cells in culture provoke telomeric overhang loss; moreover, the erosion of the telomeric overhang observed during replicative senescence may be the consequence of the cumulative stress experienced by cells during extended culture in vitro.
Our results are the first identification of a specific molecular alteration that occurs at the telomere in association with senescence. Previous studies have suggested that the telomeric overhang is an essential component of telomere structure17,18,19, and we believe that its erosion reflects the disruption of this nucleoprotein structure. Accordingly, we propose that overhang loss, rather than shortening of overall telomere length, is the molecular signal that triggers senescence. Erosion of the telomeric overhang would be expected to cause collapse of a structure such as the T-loop, to affect telomere-binding proteins and to cause exposure or 'uncapping' of the telomere end17. Alternatively, disruption of the nucleoprotein structure could lead to exposure of the telomeric overhang and to its subsequent erosion. Each of these events could in turn cause the activation of the p53 and Rb pathways, leading to senescence. Our findings thus identify a potential molecular trigger for senescence and challenge the current paradigm that telomere shortening is the molecular clock that limits replicative lifespan.
Methods
T-OLA analysis.
We carried out the T-OLA assay as described20. Briefly, we extracted genomic DNA by standard cell lysis, proteinase K treatment, phenol and chloroform extraction and RNaseA treatment. We used 5 μg of genomic DNA per assay in a 20-μl reaction volume containing 0.5 pmol 32P-end-labeled oligonucleotide of the sequence (CCCTAA)4. We used oligonucleotides of the sequence (TTAGGG)4 to detect the C-rich strand and of the sequence (CCCTTA)4 as a mismatch control. We carried out hybridization for 12–15 h at 50 °C followed by ligation using 20 units of Taq DNA ligase (New England Biolabs) at 50 °C for 5 h. After ligation, we precipitated and dried the reactions, resuspended products in water and denatured them in a formamide-based loading buffer. We separated products on 5% acrylamide, 6 M urea gels. To ensure equal DNA loading of T-OLA gels, we used 10 ng of every T-OLA sample as template for quantitative PCR reaction for the genomic GAPD gene. Primer sequences are available on request. In the reconstituted system, we used 2, 20 or 200 pg of a 200-bp fragment or 5, 50 or 500 pg of a 350-bp fragment, both containing telomeric repeats, as templates together with 5 μg of Saccharomyces cerevisiae genomic DNA. We carried out enzyme treatments of genomic DNA as follows: 0.25μg μl−1 of genomic DNA was treated with 0.6 units μl−1 T7 Gene 6 exonuclease (Roche) for 25 min at 37 °C, with 0.3 units μl−1 Bal31 nuclease (New England Biolabs) for 25 min at 30 °C or 1 unit μl−1 Exonuclease III (USB) for 30 min at 37 °C. We treated 0.05 μg μl−1 of genomic DNA with 1 unit μl−1 Exonuclease I (USB) for 24 h at 37 °C or 1 unit μg−1 Klenow DNA polymerase I (New England Biolabs) in the presence of 33 μM dNTPs for 25 min.
TRF Southern-blot analysis.
We digested 3 μg of total genomic DNA for 16 h with RsaI and HinfI and separated it on a 0.7% Tris–borate–EDTA agarose gel. We then dried gels at 63 °C for 50 min and prehybridized them in 5× Denhardt's solution, 5× sodium chloride/sodium citrate buffer, 0.1% SDS and 20 mM NaH2PO4 for 5 h at 55 °C. We added 32P-labeled probe and hybridized for 15 h. We washed gels overnight in 2× sodium chloride/sodium citrate buffer and 0.1% SDS at 55 °C and exposed them to film. For denatured gel hybridization, we incubated gels in 1.5 M NaCl and 0.5 N NaOH and then neutralized them in 3 M NaCl and 0.5 M Tris, pH 7.4, before hybridization.
Cell culture and media.
We grew BJ fibroblasts in a 4:1 mixture of Dulbecco's modified Eagle medium and M199 medium containing 15% fetal calf serum and grew MRC5 fibroblasts in Dulbecco's modified Eagle medium containing 10% fetal calf serum. Cells were split 1:4 or 1:8 on reaching confluency. We introduced TERT and T-Ag into the cells as previously described26. For contact inhibition, we grew BJ cells to confluency and held them for 4 d or 4 wk, replacing medium every 2 d. For stress exposures, we exposed BJ cells to 6 Gy or 12 Gy γ–irradiation or treated them with the following drugs for 24 h: 6 μg ml−1 doxorubicin, 100 mM cisplatin, 150 mM hydrogen peroxide, 25 mM methyl-nitro-nitroso-guanidine, 1 μg ml−1 cycloheximide, 2 μg ml−1 actinomycin D or 2 mM hydroxyurea. For hyperoxic growth conditions, we grew cells for 2 wk in 40% oxygen. For nutrient starvation, we grew cells in medium deficient of glucose or deficient in leucine and glutamine for 48 h. None of the treatments resulted in a senescence-like phenotype, as determined by morphology and the absence of senescence-associated β-galactosidase staining (data not shown). We carried out senescence-associated β-galactosidase staining as previously described27.
Densitometric analysis.
We processed scanned images using NIH Image software to assess signal intensity of each T-OLA product. To correct for the non-Gaussian skewness of the data, we log-transformed the relative intensity values and calculated geometric mean intensities of duplicate products using modified analysis of variance28. We tested values against a null hypothesis where the product intensities of each sample are equal to those of the first sample, allowing for a trend in mean intensity from small to large products. Estimated contrasts between samples were transformed to relative changes and confidence intervals.
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Acknowledgements
We would like to thank E. D'Ambrosio for helpful advice regarding T-OLA and for sharing unpublished results, F. Barany for repeated helpful advice, T. de Lange and J. Griffith for plasmids and K. Yates, Y. Dor, J. Yang, R. Watnick, P. Gupta, H. Vaziri, S. Dessain and other members of R.A.W.'s laboratory for helpful comments, discussion and critical review of the manuscript. This work was supported by Merck/MIT (R.A.W.), the US National Cancer Institute (R.A.W.), an American Association for Cancer Research Postdoctoral Fellowship (S.A.S.), an EMBO Long-Term Fellowship (I.B.), the Dana Farber Cancer Institute (V.J.C.), the US National Cancer Institute Howard Temin award (W.C.H.), a Doris Duke Charitable Foundation Clinical Scientist Development Award (W.C.H.) and a Kimmel Scholar Award (W.C.H.). R.A.W. is an American Cancer Society Research Professor and a Daniel K. Ludwig Cancer Research Professor.
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Stewart, S., Ben-Porath, I., Carey, V. et al. Erosion of the telomeric single-strand overhang at replicative senescence. Nat Genet 33, 492–496 (2003). https://doi.org/10.1038/ng1127
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DOI: https://doi.org/10.1038/ng1127
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