Literature DB >> 17292509

Effects of fibroblasts and microenvironment on epidermal regeneration and tissue function in long-term skin equivalents.

Karsten Boehnke1, Nicolae Mirancea, Alessandra Pavesio, Norbert E Fusenig, Petra Boukamp, Hans-Jürgen Stark.   

Abstract

In vitro generated skin models find growing interest as promising tools in basic research and clinical application in regenerative medicine. Here, we present further details of an improved long-term skin equivalent (SE) enabling mechanistic studies on skin reconstruction and epidermal function. Growth conditions of fibroblasts in a 3D scaffold were analysed to optimise the dermal microenvironment by providing an authentic dermal matrix for regular tissue reconstruction and function of cocultured keratinocytes. These SEs demonstrate sustained epidermal viability - over 12 weeks - with regular differentiation as substantiated by in vivo-like patterns of all differentiation products, exemplified here by the cornified envelope components loricrin and repetin. The continuous expression of all major tight junction components in the granular layer, shown here for ZO-1 in coherence with the presence of epidermal barrier lipids, and ultrastructural accumulation of lamellar bodies, collectively indicate proper epidermal barrier structures. Remarkably, cocultured keratinocytes exerted an ongoing proliferation-stimulating effect on fibroblasts colonising the scaffold comparable to a cocktail of fibroblast growth factors. Consequently, precultivation of dermal equivalents (DEs) in basal or growth factor-enriched media had only minor effects on the quality of epidermal regeneration in cocultures. As to the role of fibroblast numbers, complete absence of dermal cells resulted in atrophic epithelia but the effect of cell numbers as low as 5 x 10(4)cells/cm(2) on epidermal tissue quality equalled that of the standard density (2 x 10(5)cells/cm(2)). Surprisingly, precultivation of fibroblasts in the DEs for 7 days (standard) showed no better effect on epidermal tissue reformation as compared to 2 days whereas a precultivation period of 14 days resulted in atrophic epidermal and dermal tissue development. These data demonstrate, (i) the strict dependence of epidermal tissue regeneration on the presence of fibroblasts, (ii) the mutual keratinocyte-fibroblast interactions for cell proliferation and organogenesis, and (iii) the importance of the proper microenvironment for epidermal tissue function and supposedly for establishment of a stem cell niche in vitro.

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Year:  2007        PMID: 17292509     DOI: 10.1016/j.ejcb.2006.12.005

Source DB:  PubMed          Journal:  Eur J Cell Biol        ISSN: 0171-9335            Impact factor:   4.492


  40 in total

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5.  Tissue microenvironment initiates an immune response to structural components of Staphylococcus aureus.

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7.  Bryostatin and its synthetic analog, picolog rescue dermal fibroblasts from prolonged stress and contribute to survival and rejuvenation of human skin equivalents.

Authors:  Tapan K Khan; Paul A Wender; Daniel L Alkon
Journal:  J Cell Physiol       Date:  2017-07-11       Impact factor: 6.384

8.  Natural corneal cell-based microenvironment as prerequisite for balanced 3D corneal epithelial morphogenesis: a promising animal experiment-abandoning tool in ophthalmology.

Authors:  Simon Schulz; David Beck; Dougal Laird; Thorsten Steinberg; Pascal Tomakidi; Thomas Reinhard; Philipp Eberwein
Journal:  Tissue Eng Part C Methods       Date:  2013-09-09       Impact factor: 3.056

9.  Organotypic modelling as a means of investigating epithelial-stromal interactions during tumourigenesis.

Authors:  Athina-Myrto Chioni; Richard Grose
Journal:  Fibrogenesis Tissue Repair       Date:  2008-12-11

10.  Aging alters functionally human dermal papillary fibroblasts but not reticular fibroblasts: a new view of skin morphogenesis and aging.

Authors:  Solène Mine; Nicolas O Fortunel; Hervé Pageon; Daniel Asselineau
Journal:  PLoS One       Date:  2008-12-30       Impact factor: 3.240

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