Towards the development of a simplified long‐term organ culture method for human scalp skin and its appendages under serum‐free conditions

Zhang, Lu; Hasse, Sybille; Bodó, Enikő; Rosé, Christian; Funk, Wolfgang; Paus, Ralf

doi:10.1111/j.1600-0625.2006.00510.x

Cited by 123 publications

(168 citation statements)

References 36 publications

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“…Skin thickness varied based on anatomic region and individual characteristics of the donor (,1 mm for eyelids, 1-2 mm for breast and inguinal, 2-5 mm for abdomen and thigh skin). Cylindrical skin explants, 4 mm in diameter (12.5 mm 2 ), were prepared with a sterile biopsy tool and immediately placed in prewarmed Williams' E medium supplemented with insulin (10 mg·ml -1 ), hydrocortisone (10 ng·ml -1 ), and penicillin-streptomycinglutamine (100 U·ml -1 of penicillin; 100 mg·ml -1 of streptomycin; 2 mM L-glutamine) (Lu et al, 2007). Medium pH value was 7.4, culturing temperature was 37°C, incubator humidity was 90%, and CO 2 content was 5%.…”

Section: Skin Explants Culturementioning

confidence: 99%

Phase II Metabolism in Human Skin: Skin Explants Show Full Coverage for Glucuronidation, Sulfation,N-Acetylation, Catechol Methylation, and Glutathione Conjugation

et al. 2014

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Although skin is the largest organ of the human body, cutaneous drug metabolism is often overlooked, and existing experimental models are insufficiently validated. This proof-of-concept study investigated phase II biotransformation of 11 test substrates in fresh full-thickness human skin explants, a model containing all skin cell types. Results show that skin explants have significant capacity for glucuronidation, sulfation, N-acetylation, catechol methylation, and glutathione conjugation. Novel skin metabolites were identified, including acyl glucuronides of indomethacin and diclofenac, glucuronides of 17b-estradiol, N-acetylprocainamide, and methoxy derivatives of 4-nitrocatechol and 2,3-dihydroxynaphthalene. Measured activities for 10 mM substrate incubations spanned a 1000-fold: from the highest 4.758 pmol·mg skin ·h -1 for 17b-estradiol 17-glucuronidation. Interindividual variability was 1.4-to 13.0-fold, the highest being 4-methylumbelliferone and diclofenac glucuronidation. Reaction rates were generally linear up to 4 hours, although 24-hour incubations enabled detection of metabolites in trace amounts. All reactions were unaffected by the inclusion of cosubstrates, and freezing of the fresh skin led to loss of glucuronidation activity. The predicted whole-skin intrinsic metabolic clearances were significantly lower compared with corresponding whole-liver intrinsic clearances, suggesting a relatively limited contribution of the skin to the body's total systemic phase II enzymemediated metabolic clearance. Nevertheless, the fresh full-thickness skin explants represent a suitable model to study cutaneous phase II metabolism not only in drug elimination but also in toxicity, as formation of acyl glucuronides and sulfate conjugates could play a role in skin adverse reactions.

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Section: Skin Explants Culturementioning

confidence: 99%

Phase II Metabolism in Human Skin: Skin Explants Show Full Coverage for Glucuronidation, Sulfation,N-Acetylation, Catechol Methylation, and Glutathione Conjugation

et al. 2014

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“…in atopic (HFs), the follicular connective tissue sheath (CTS) 10,11 . Therefore, we 138 hypothesized that robust mechanisms must be in place to avoid excessive angiogenesis, wound healing and hair growth 8,10,12 . Moreover, the maturation …”

Section: Introductionmentioning

confidence: 99%

“…[8][9][10][11] . HFs were first incubated overnight to adapt to culture conditions 755 after which the medium was replaced and vehicle or test substances was added.…”

mentioning

confidence: 99%

Endocannabinoids limit excessive mast cell maturation and activation in human skin

Sugawara

Bı́ró

Tsuruta

et al. 2012

Journal of Allergy and Clinical Immunology

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120

165

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“…Even in optimized conditions, HFs begin to degenerate after 20 days in culture, on average, while apoptotic cells appear approximately on day 5 [86]. HFs maintained in vitro are unable to keep cycling [87,88].…”

Section: Hair Follicle Reconstructionmentioning

confidence: 99%

Hair Follicle Reconstruction and Stem Cells

Kalabusheva¹,

Chermnykh²,

Terskikh³

et al. 2017

Hair and Scalp Disorders

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De novo hair follicle (HF) formation in embryonic skin and hair growth in postnatal skin are the result of epithelial-mesenchymal interactions between specialized mesenchymal dermal papilla (DP) and epithelial stem cells that give rise to hairs. Adult HF is a valuable source of diferent lineages of stem cells (SCs) with morphogenetic potential. Epithelial stem cells are residing in the special compartment of HF (the bulge) and can be mobilized to regenerate the new follicle with each hair cycle and to reepithelialize epidermis during wound repair. This review summarizes the current knowledge on key characteristics of HF SC populations in terms of regenerative potential. General biological principles that govern the mesenchymal-epithelial interactions within the HF and the signaling pathways that control HF development are discussed. The main focus is on recent approaches to reconstruct folliculogenesis in vitro and perspectives of the tissue engineering in alopecia therapy.

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Towards the development of a simplified long‐term organ culture method for human scalp skin and its appendages under serum‐free conditions

Cited by 123 publications

References 36 publications

Phase II Metabolism in Human Skin: Skin Explants Show Full Coverage for Glucuronidation, Sulfation,N-Acetylation, Catechol Methylation, and Glutathione Conjugation

Phase II Metabolism in Human Skin: Skin Explants Show Full Coverage for Glucuronidation, Sulfation,N-Acetylation, Catechol Methylation, and Glutathione Conjugation

Endocannabinoids limit excessive mast cell maturation and activation in human skin

Hair Follicle Reconstruction and Stem Cells

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