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Featured researches published by Melanie Giesen.


Journal of Investigative Dermatology | 2014

Hypothalamic-pituitary-thyroid axis hormones stimulate mitochondrial function and biogenesis in human hair follicles

Silvia Vidali; Jana Knuever; J. Lerchner; Melanie Giesen; Tamás Bíró; Matthias Klinger; Barbara Kofler; Wolfgang Funk; Burkhard Poeggeler; Ralf Paus

Thyroid hormones regulate mitochondrial function. As other hypothalamic-pituitary-thyroid (HPT) axis hormones, i.e., thyrotropin-releasing hormone (TRH) and thyrotropin (TSH), are expressed in human hair follicles (HFs) and regulate mitochondrial function in human epidermis, we investigated in organ-cultured human scalp HFs whether TRH (30 nM), TSH (10 mU ml(-1)), thyroxine (T4) (100 nM), and triiodothyronine (T3) (100 pM) alter intrafollicular mitochondrial energy metabolism. All HPT-axis members increased gene and protein expression of mitochondrial-encoded subunit 1 of cytochrome c oxidase (MTCO1), a subunit of respiratory chain complex IV, mitochondrial transcription factor A (TFAM), and Porin. All hormones also stimulated intrafollicular complex I/IV activity and mitochondrial biogenesis. The TSH effects on MTCO1, TFAM, and porin could be abolished by K1-70, a TSH-receptor antagonist, suggesting a TSH receptor-mediated action. Notably, as measured by calorimetry, T3 and TSH increased follicular heat production, whereas T3/T4 and TRH stimulated ATP production in cultured HF keratinocytes. HPT-axis hormones did not increase reactive oxygen species (ROS) production. Rather, T3 and T4 reduced ROS formation, and all tested HPT-axis hormones increased the transcription of ROS scavengers (catalase, superoxide dismutase 2) in HF keratinocytes. Thus, mitochondrial biology, energy metabolism, and redox state of human HFs are subject to profound (neuro-)endocrine regulation by HPT-axis hormones. The neuroendocrine control of mitochondrial biology in a complex human mini-organ revealed here may be therapeutically exploitable.


Experimental Dermatology | 2011

Ageing processes influence keratin and KAP expression in human hair follicles

Melanie Giesen; Sabine Gruedl; Olaf Holtkoetter; Guido Fuhrmann; Andrea Koerner; Dirk Petersohn

Abstract:  In many cultures, a youthful look is strictly linked to strong and healthy hair. Source of the hair fibre is the hair follicle, a highly specialized skin appendage. Biological alterations because of intrinsic or extrinsic stimuli can destabilize this perfectly organized system, thus effecting hair growth or metabolism. Also, ageing could be characterized as a disturbance in this well‐balanced machinery. Albeit the predominant symptom of hair ageing, greying, is addressed in a plurality of research activities, further age‐related changes, e.g. related to hair structure, remain obscure. Therefore, we characterized hair follicles of two volunteer panels (below 25 years, above 50 years) on the molecular level, especially focussing on alterations influencing gene expression of keratins and keratin‐associated proteins. We showed that concordantly to other biological systems the hair follicle undergoes several modifications during the ageing process associated among others with a significant decline in these structural proteins. Providing strategies to fight against these age‐related changes is a challenge for hair science.


Experimental Dermatology | 2016

A three-dimensional skin equivalent reflecting some aspects of in vivo aged skin.

Johanna Diekmann; Lirija Alili; Okka Scholz; Melanie Giesen; Olaf Holtkötter; Peter Brenneisen

Human skin undergoes morphological, biochemical and functional modifications during the ageing process. This study was designed to produce a 3‐dimensional (3D) skin equivalent in vitro reflecting some aspects of in vivo aged skin. Reconstructed skin was generated by co‐culturing skin fibroblasts and keratinocytes on a collagen–glycosaminoglycan–chitosan scaffold, and ageing was induced by the exposition of fibroblasts to Mitomycin‐C (MMC). Recently published data showed that MMC treatment resulted in a drug‐induced accelerated senescence (DIAS) in human dermal fibroblast cultures. Next to established ageing markers, histological changes were analysed in comparison with in vivo aged skin. In aged epidermis, the filaggrin expression is reduced in vivo and in vitro. Furthermore, in dermal tissue, the amount of elastin and collagen is lowered in aged skin in vivo as well as after the treatment of 3D skin equivalents with MMC in vitro. Our results show histological signs and some aspects of ageing in a 3D skin equivalent in vitro, which mimics aged skin in vivo.


PLOS ONE | 2017

A novel organotypic 3D sweat gland model with physiological functionality

Patricia Klaka; Sabine Grüdl; Bernhard Banowski; Melanie Giesen; Andrea Sättler; Peter Proksch; Thomas Welss; Thomas Förster

Dysregulated human eccrine sweat glands can negatively impact the quality-of-life of people suffering from disorders like hyperhidrosis. Inability of sweating can even result in serious health effects in humans affected by anhidrosis. The underlying mechanisms must be elucidated and a reliable in vitro test system for drug screening must be developed. Here we describe a novel organotypic three-dimensional (3D) sweat gland model made of primary human eccrine sweat gland cells. Initial experiments revealed that eccrine sweat gland cells in a two-dimensional (2D) culture lose typical physiological markers. To resemble the in vivo situation as close as possible, we applied the hanging drop cultivation technology regaining most of the markers when cultured in its natural spherical environment. To compare the organotypic 3D sweat gland model versus human sweat glands in vivo, we compared markers relevant for the eccrine sweat gland using transcriptomic and proteomic analysis. Comparing the marker profile, a high in vitro-in vivo correlation was shown. Carcinoembryonic antigen-related cell adhesion molecule 5 (CEACAM5), muscarinic acetylcholine receptor M3 (CHRM3), Na+-K+-Cl- cotransporter 1 (NKCC1), calcium-activated chloride channel anoctamin-1 (ANO1/TMEM16A), and aquaporin-5 (AQP5) are found at significant expression levels in the 3D model. Moreover, cholinergic stimulation with acetylcholine or pilocarpine leads to calcium influx monitored in a calcium flux assay. Cholinergic stimulation cannot be achieved with the sweat gland cell line NCL-SG3 used as a sweat gland model system. Our results show clear benefits of the organotypic 3D sweat gland model versus 2D cultures in terms of the expression of essential eccrine sweat gland key regulators and in the physiological response to stimulation. Taken together, this novel organotypic 3D sweat gland model shows a good in vitro-in vivo correlation and is an appropriate alternative for screening of potential bioactives regulating the sweat mechanism.


Archive | 2004

Skin/hair equivalent with reconstructed papillae

Kordula Schlotmann; Thomas Gassenmeier; Ralf Paus; Melanie Giesen; Dirk Petersohn


Archive | 2008

Agent containing l-carnitine or l-carnitine derivatives and at least one other specific substance

Melanie Giesen; Klaus Schroeder; Dirk Petersohn


Archive | 2007

Cosmetic composition comprising purine and/or a purine derivative and taurine

Thorsten Knappe; Helen Walter; Thomas Dr. Weiss; Zur Wiesche Erik Schulze; Melanie Giesen; Philipp Spuhler


Archive | 2006

Method for conducting extracorporeal analysis of hair follicle cells

Melanie Giesen; Dirk Petersohn; Kordula Schlotmann; Zur Wiesche Erik Schulze; Elisabeth Poppe


Journal of Investigative Dermatology | 2016

Thyroid Hormones Enhance Mitochondrial Function in Human Epidermis

Silvia Vidali; J. Chéret; Melanie Giesen; Swantje Haeger; M. Alam; Rachel E.B. Watson; Abigail K. Langton; Matthias Klinger; Jana Knuever; Wolfgang Funk; Barbara Kofler; Ralf Paus


Archive | 2007

Hair-treatment compositions comprising quercetin and use thereof to revitalize hair

Thomas Welss; Melanie Giesen; Zur Wiesche Erik Schulze; Volker Scheunemann

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