Integrated control of growth and differentiation of normal human prokeratinocytes cultured in serum‐free medium: Clonal analyses, growth kinetics, and cell cycle studies

Wille, John J.; Pittelkow, Mark R.; Shipley, Gary D.; Scott, Robert E.

doi:10.1002/jcp.1041210106

Cited by 387 publications

(255 citation statements)

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“…An induction of MDM2 preceded that of p53, and occurred when an increase of cellular size started to become evident (see 24 h, Figure 3b). p53 and MDM2 expression during spontaneous keratinocyte differentiation Primary keratinocytes do not stratify when cultured in a de®ned serum-free low calcium medium (DKSFM) in the absence of a feeder layer but instead, they form a monolayer of basal-like proliferative cells (Hennings et al, 1980;Wille et al, 1984). However, terminal di erentiation is not suppressed and a proportion of cells within this monolayer express involucrin and eventually shed into the culture medium (Drozdo and Pledger, 1993;Watt and Green, 1982; Figure 4; unpublished results).…”

Section: Kinetics Of Expression Of P53 and Mdm2 During Suspension-indmentioning

confidence: 99%

Switch from p53 to MDM2 as differentiating human keratinocytes lose their proliferative potential and increase in cellular size

et al. 2000

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p53 transcription factor is mutated in most skin cell carcinomas and in more than 50% of all human malignancies. One of its transcriptional targets is MDM2, which in turn down-regulates p53. The role of the p53/MDM2 regulatory loop upon genotoxic stress is well documented, but less is known about its role in normal tissue homeostasis. We have explored this pathway during the di erent transitions of the human epidermal di erentiation programme and after isolating stem cells, transit amplifying cells or di erentiating cells from epidermis. Maximum expression of p53 was found in proliferating keratinocytes. A striking and transient induction of MDM2 and a down-modulation of p53 characterized the transition from proliferation to di erentiation in primary human keratinocytes. These changes were delayed in late di erentiating carcinoma cells, and were clearly di erent in suspended primary ®broblasts. Interestingly, these changes correlated with an increase in cell size, at the time of irreversible commitment to di erentiation. Induction of MDM2 was also associated with suppression of proliferation in normal, or hyperproliferative, psoriatic epidermis. Moreover, both proteins were induced as keratinocytes were driven to leave the stem cell compartment by c-Myc activation. Overall, our results show a critical regulation of the p53/MDM2 pathway at the epidermal transition from proliferation to di erentiation.

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Section: Kinetics Of Expression Of P53 and Mdm2 During Suspension-indmentioning

confidence: 99%

Switch from p53 to MDM2 as differentiating human keratinocytes lose their proliferative potential and increase in cellular size

et al. 2000

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“…In contrast, tracheobronchial epithelial and human epidermal cells exhibit optimal growth at calcium concentrations > 100 ,4M (33,43,84,85) and maintain a high colony-forming efficiency. However, high calcium does induce a reversible morphological change in these cells (33,43,84,85) Transforming Growth Factor ( Transforming growth factor p (TGF-p) is a polypeptide hormone that is expressed and released by many normal and neoplastic cells (123,124). It consists of two 12 kD chains linked by disulfide bonds and is synthesized as part of a larger secretory precursor (123).…”

Section: Role Of Calciummentioning

confidence: 96%

Multistep Process of Squamous Differentiation in Tracheobronchial Epithelial Cells In Vitro: Analogy with Epidermal Differentiation

Jetten¹

1989

Environmental Health Perspectives

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The lung, in particular the bronchial epithelium, is a major site for tumor formation in humans. Environmental factors, such as cigarette smoke, in conjunction with genetic factors are important determinants in this disease. Malignant cells exhibit alterations in their control of proliferation and differentiation. It is believed that the acquisition of defects in the regulation of these processes is important in the process of carcinogenesis. A clear insight into the basic mechanisms of the regulation of proliferation and differentiation is required to understand the molecular mechanisms involved in tumor development and in other pathological conditions. Studies using in vitro cell culture systems of tracheobronchial epithelial cells provide useful models in which to study the regulation of differentiation and proliferation. The clonogenic cells derived from the treacheobronchial epithelium are pluripotent: They have self-renewal capacity and can differentiate along either a normal, mucosecretory, or a squamous cell pathway. Squamous differentiation in tracheobronchial epithelial cells has many morphological, biochemical, and regulatory properties in common with epidermal differentiation. This pathway of differentiation is a multistep process consisting of at least three stages. In the initial stage, cells become committed to terminal cell division. This is followed by the expression of the squamous differentiated phenotype and finally cornification. Various factors, such as several growth factors, retinoids, calcium ions, and phorbol esters, regulate the program of differentiation at different stages. Studies have indicated that the controls of proliferation and differentiation are interrelated. Cell lines established from tracheobronchial epithelial cells expressing SV40 large T-antigen, as well as carcinoma cell lines, exhibit altered responses to growth and differentiation regulatory factors Alterations in the commitment to terminal cell division must be a crucial step in the transition of a normal to a malignant cell.

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“…Different culture media have been used to improve cell culture yield and the viability of keratinocytes from humans, mice and adult pigs [2,6,[20][21][22], but no medium has been described yet for keratinocytes isolated from neonatal pigs.…”

Section: Medium-dependent Proliferation and Viability Of Keratinocytesmentioning

confidence: 99%

“…In vitro, keratinocyte differentiation has been successfully induced by several factors, such as osmotic stress, growth factors, high calcium concentrations, or serum supplementation [16,22,23,27,46]. To investigate whether the keratinocytes isolated from piglets retain the ability to differentiate in vitro after the isolation procedure, normal keratinocyte growth medium (EKGM) was replaced with a differentiation medium.…”

Section: Effect Of Calcium and Serum On Cell Differentiation Of Keratmentioning

confidence: 99%

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Isolation and cultivation of primary keratinocytes from piglet skin for compartmentalized co-culture with dorsal root ganglion neurons

Ponce

Heintz

Schäfer

et al. 2017

JCB

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Abstract. Keratinocytes are the main cell population in the epidermis, where they coexist with a variety of other cell types. Their successful isolation and cultivation have afforded opportunities to study epidermal functions. Human keratinocytes have been studied most extensively, but their source is limited by the skin supply. In a previous work, we developed an in vitro co-culture model of porcine keratinocytes with porcine sensory neurites to investigate functional interaction. However, a detailed description of the isolation of porcine keratinocytes and their culture conditions has not been given in detail. Here, we present the isolation procedure and a characterization of keratinocytes derived from new-born piglets, using simple assays based on conventional and fluorescence microscopy. Media, coating substrates and plating densities were tested with respect to cell viability, proliferation and morphology. Growing keratinocytes in EpiLife keratinocyte growth medium (EKGM) on human collagen type I substrate was best to support proliferation. The minimum plated density was 500 viable cells/cm 2 for primary and 1000 viable cells/cm 2 for subcultured cells. Population doubling (PD) and generation time (tg) depended on the plating densities. Keratinocytes seeded at a density of 5000 viable cells/cm 2 had a PD of 4.36 ± 0.60 per passage and tg of 1.69 ± 0.24 days. Our results show that the optimal isolation and culture conditions for keratinocytes from piglets differ from those for keratinocytes from adult pigs and humans. Thus, the information obtained from the characterization allowed the performance and optimization of a co-culture and contributes to further investigations in epidermal homeostasis and cutaneous sensation.

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Integrated control of growth and differentiation of normal human prokeratinocytes cultured in serum‐free medium: Clonal analyses, growth kinetics, and cell cycle studies

Cited by 387 publications

References 50 publications

Switch from p53 to MDM2 as differentiating human keratinocytes lose their proliferative potential and increase in cellular size

Switch from p53 to MDM2 as differentiating human keratinocytes lose their proliferative potential and increase in cellular size

Multistep Process of Squamous Differentiation in Tracheobronchial Epithelial Cells In Vitro: Analogy with Epidermal Differentiation

Isolation and cultivation of primary keratinocytes from piglet skin for compartmentalized co-culture with dorsal root ganglion neurons

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