Human fibroblast replicative senescence can occur in the absence of extensive cell division and short telomeres

Munro, June; Steeghs, Karen; Morrison, Vivienne; Ireland, H. Elyse; Parkinson, Eric Kenneth

doi:10.1038/sj.onc.1204460

Cited by 73 publications

(71 citation statements)

References 47 publications

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“…The high molecular weight smears in the D17 experiment (particularly lanes 3 and 7) are often seen in keratinocyte TRF blots (Gordon et al, 2002) and are probably due to small amounts of 3T3 DNA contamination that gave a disproportionately high signal because mouse TRFs are 10-25 more abundant than in our human oral cultures. TRF measurements were carried out as described by Munro et al (2001), except that the blot was hybridized with a radiolabelled oligonucleotide probe (TTAGGG) 3 at 421C and subsequently washed in 6 Â SSC/1% SDS at 421C Figure 2 Telomerase activity in D30 and D17 cultures before and after infection with the hTERT expression vector. D30 cells were infected with hTERT or empty vector retroviruses at 9 PDs and analysed as soon as sufficient cells were available; D17 cells were infected at 39 PDs and analysed at 58 PDs.…”

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confidence: 99%

Senescing oral dysplasias are not immortalized by ectopic expression of hTERT alone without other molecular changes, such as loss of INK4A and/or retinoic acid receptor-β: but p53 mutations are not necessarily required

et al. 2003

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Senescing oral dysplasias are not immortalized by ectopic expression of hTERT alone without other molecular changes, such as loss of INK4A and/or retinoic acid receptor-β: but p53 mutations are not necessarily required

et al. 2003

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“…The authors referred to this mode of cellular ageing as chronological lifespan (CLS). We and others have shown that quiescent human fibroblasts cultured for a long duration were unable to proliferate following replating at a lower cell density (Allsopp et al 1995;Munro et al 2001;Sarsour et al 2005;Sitte et al 1998). We observed that quiescent fibroblasts lost their proliferative capacity (measured as percentage of S phase at 48 h following replating of cells at a lower cell density) beginning from 30 days of quiescence; a maximal drop in S phase percentage was observed in cells replated from 60 days of quiescence (Sarsour et al 2005).…”

Section: Introductionmentioning

confidence: 68%

“…Although HT is an antioxidant, it can initially act as a prooxidant leading to the generation of superoxide and activation of MnSOD expression. Previous literature showed that long duration of quiescence resulted in a significant loss in the proliferative capacity of NHFs (Munro et al 2001;Sarsour et al 2005;Sitte et al 1998). We used contact-inhibited quiescent, but metabolically active cultures to study the effects of HT on CLS of NHFs.…”

Section: Discussionmentioning

confidence: 98%

“…c HT generates free radicals: in the presence of hydrogen peroxide, peroxidases oxidize HT to its semiquinone radical, which in turn leads to the formation of superoxide and quinone. (Munro et al 2001) where the authors report loss of 15-25 population doublings in long-term quiescent cultures of normal human fibroblasts. This loss in population doublings was associated with approximately 94% of the cells exiting the cell cycle permanently.…”

Section: Discussionmentioning

confidence: 99%

“…The decrease in S phase was not due to cell death or changes in telomerase activity. Mid-lifespan fibroblasts kept in quiescence for 7-12 weeks lost their proliferative capacity, yet there were no detectable shortening of telomere (Allsopp et al 1995;Munro et al 2001;Sitte et al 1998). Results from these previous studies suggest the presence of telomere-independent pathways that influence cellular lifespan.…”

Section: Introductionmentioning

confidence: 86%

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MnSOD activity regulates hydroxytyrosol-induced extension of chronological lifespan

Sarsour

Kumar

Kalen

et al. 2011

AGE

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Chronological lifespan (CLS) is defined as the duration of quiescence in which normal cells retain the capacity to reenter the proliferative cycle. This study investigates whether hydroxytyrosol (HT), a naturally occurring polyphenol found in olives, extends CLS in normal human fibroblasts (NHFs). Quiescent NHFs cultured for a long duration (30-60 days) lose their capacity to repopulate. Approximately 60% of these cells exit the cell cycle permanently; a significant increase in the doubling time of the cell population was observed. CLS was extended in quiescent NHFs that were cultured in the presence of HT for 30-60 days. HT-induced extension of CLS was associated with an approximately 3-fold increase in manganese superoxide dismutase (MnSOD) activity while there was no change in copper-zinc superoxide dismutase, catalase, or glutathione peroxidase protein levels. Quiescent NHFs overexpressing a dominant-negative mutant form of MnSOD failed to extend CLS. HT suppressed ageassociated increase in mitochondrial ROS levels. Results from spectroscopy assays indicate that HT in the presence of peroxidases can undergo catechol-semiquinone-quinone redox cycling generating superoxide, which in a cellular context can activate the antioxidant system, e.g., MnSOD expression. These results demonstrate that HT extends CLS by increasing MnSOD activity and decreasing age-associated mitochondrial reactive oxygen species accumulation.

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Tissue‐Engineered Cochlear Fibrosis Model Links Complex Impedance to Fibrosis Formation for Cochlear Implant Patients

Rijk

Boys

Roberts

et al. 2023

Adv Healthcare Materials

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Cochlear implants are a life‐changing technology for those with severe sensorineural hearing loss, partially restoring hearing through direct electrical stimulation of the auditory nerve. However, they are known to elicit an immune response resulting in fibrotic tissue formation in the cochlea that is linked to residual hearing loss and suboptimal outcomes. Intracochlear fibrosis is difficult to track without postmortem histology, and no specific electrical marker for fibrosis exists. In this study, a tissue‐engineered model of cochlear fibrosis is developed following implant placement to examine the electrical characteristics associated with fibrotic tissue formation around electrodes. The model is characterized using electrochemical impedance spectroscopy and an increase in the resistance and a decrease in capacitance of the tissue using a representative circuit are found. This result informs a new marker of fibrosis progression over time that is extractable from voltage waveform responses, which can be directly measured in cochlear implant patients. This marker is tested in a small sample size of recently implanted cochlear implant patients, showing a significant increase over two postoperative timepoints. Using this system, complex impedance is demonstrated as a marker of fibrosis progression that is directly measurable from cochlear implants to enable real‐time tracking of fibrosis formation in patients, creating opportunities for earlier treatment intervention to improve cochlear implant efficacy.

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Human fibroblast replicative senescence can occur in the absence of extensive cell division and short telomeres

Cited by 73 publications

References 47 publications

Senescing oral dysplasias are not immortalized by ectopic expression of hTERT alone without other molecular changes, such as loss of INK4A and/or retinoic acid receptor-β: but p53 mutations are not necessarily required

Senescing oral dysplasias are not immortalized by ectopic expression of hTERT alone without other molecular changes, such as loss of INK4A and/or retinoic acid receptor-β: but p53 mutations are not necessarily required

MnSOD activity regulates hydroxytyrosol-induced extension of chronological lifespan

Tissue‐Engineered Cochlear Fibrosis Model Links Complex Impedance to Fibrosis Formation for Cochlear Implant Patients

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