Efeitos dos inibidores da enzima ácido graxo sintase sobre apoptose e função mitocondrial de células não tumorigênicas / Fatty acid synthase inhibitors effects on apoptosis and mitochondrial function in non tumorigenic cells

Rossato, Franco Aparecido, 1984-

24 August 2018

Orientadores: Anibal Eugênio Vercesi, Karina Gottardelo Zecchin / Texto em português e inglês / Tese (doutorado) - Universidade Estadual de Campinas, Faculdade de Ciências Médicas / Made available in DSpace on 2018-08-24T16:40:04Z (GMT). No. of bitstreams: 1 Rossato_FrancoAparecido_D.pdf: 7526681 bytes, checksum: 3768c017da7bde02ddd95e8e41881438 (MD5) Previous issue date: 2014 / Resumo: Recentemente mostramos que os inibidores da enzima ácido graxo sintase (FASN - EC 2.3.1.85), cerulenina e orlistat, reduzem a proliferação e induzem apoptose em células B16-F10 de melanoma murino via mecanismos mitocondriais. Neste presente estudo investigamos os efeitos desses inibidores de FASN em linhagem celular não-tumorigênica derivada de melanoblastos de camundongos (melan-a). O tratamento in vitro de células melan-a com 5 µg/mL de cerulenina ou com 30 µM de orlistat inibiu a proliferação celular, com acúmulo da proteína supressora de tumor p21WAF1/Cip1, assim como induziu a via intrínseca da apoptose com liberação de citocromo c e ativação de caspases-3 e -9, sem ativação da caspase-8. Os inibidores de FASN não alteram o conteúdo de ácidos graxos livres nas células melan-a, verificados por espectrometria de massas, sugerindo que o tratamento com cerulenina ou orlistat induz apoptose independente da inibição desta enzima. Análise das funções da bioenergética mitocondrial das células melan-a mostraram inibição da respiração, seguido por aumento da produção de superóxido. A inibição da respiração, promovida pelo tratamento com cerulenina ou orlistat, foi restrita à oxidação de substratos ligados a NADH (39,9% DMSO x cerulenina; ou 60,8% EtOH x orlistat) e succinato (45,8% DMSO x cerulenina; ou 51,8% EtOH x orlistat), e não foi significativa quando as mitocôndrias estavam respirando com substrato do complexo IV, N,N,N',N'-tetrametil-p-fenilenodiamina. A proteção conferida pelo sequestrador de radicais livres N-acetil cisteína (NAC) sugere que a disfunção mitocondrial provocada por estes compostos está associada a estresse oxidativo e é provável que seja mediada pela ação de superóxido na cadeia respiratória nos níveis de complexos de I e II. Análise proteômica de mitocôndria dessas células também mostra alterações ligadas ao estresse oxidativo. Nossos dados em conjunto sugerem que cerulenina e orlistat induzem apoptose em células não tumorais como resultado de uma disfunção mitocondrial e de maneira independente de FASN / Abstract: We have previously reported that the fatty acid synthase (FASN) inhibitors, cerulenin or orlistat, induce apoptosis in B16-F10 mouse melanoma cells mediated by mitochondria. Here we investigate the effects of these inhibitors on the non-tumorigenic mouse cell line melan-a. Cerulenin or orlistat treatment decreased cells proliferation, accompanied by increased amounts of the tumor suppressor protein p21WAF1/Cip1, as well as induced apoptosis, but not necrosis, in melan-a cell line. Mitochondrial cytochrome c release and activation of caspases-9 and -3 were detected in melan-a-treated cells. siRNAi for FASN did not culminate in apoptosis, and FASN inhibitors treatment did not alter free fatty acids content in the non-tumorigenic cells, as verified by mass spectrometry, suggesting that cerulenin or orlistat induces apoptosis independent on FASN inhibition. Analysis of energy-linked functions of melan-a mitochondria showed inhibition of respiration followed by large stimulation of superoxide production. Respiratory inhibition after cerulenin or orlistat treatment, respectively, was restricted to the oxidation of NADH-linked substrates (39.9 or 60,8%) and succinate (45.8 or 51.8%) and was not significant when mitochondria were respiring on the complex IV substrate, N,N,N?,N?-tetramethyl-p-phenylendiamine. The protection conferred by the free radical scavenger NAC suggests that the mitochondrial dysfunction caused by these compounds is associated with oxidative stress and is mediated by the action of superoxide on the respiratory chain at the levels of complexes-I and II. Proteomic analysis of mitochondria melan-a cells also indicate major changes linked to oxidative stress. Taken together, the present results show that cerulenin or orlistat induces apoptosis in non-tumorigenic cells via mitochondrial dysfunction, independent on FASN inhibition / Doutorado / Fisiopatologia Médica / Doutor em Ciências

Melanócitos

Inibidores da síntese de ácidos graxos

Apoptose

Mitocôndria

Complexo ácido graxo sintetase

Melanocytes

Fatty acid synthesis inhibitors

Apoptosis

Mitochondria

Fatty acid synthetase complex

1-How in vivo cutaneous biometrology could demonstrate skin modifications induced by various methods. 2-In vitro evaluation of phenytoin on the morphology and activity of human primary melanocytes and in vivo repigmentation effect of topical phenytoin / 1-Comment la biométrologie cutanée in vivo peut démontrer les modifications de la peau induites par diverses méthodes d'évaluation. 2-Evaluation d'effet de la phénytoïne sur la morphologie et l'activité des mélannocytes primaires humaines in vitro et l'effet de repigmentation in vivo de la phénytoïne topique

Fanian, Ferial

14 December 2016

La Biometrogie cutanée est un nouveau spectre de différentes méthodes d'évaluation qui permettent de mesurer les différents paramètres de la peau même en cas des petites modifications. Dans la première partie de nos travaux, nous avons étudié différentes capacités de ces méthodes afin de les corréler avec d'autres données cliniques et histologiques. Ces données nous ont encouragés à découvrir de plus en plus la pigmentation de la peau qui est un peu plus compliquée que les autres paramètres. Par conséquent, sur la deuxième partie, nous nous sommes concentrés sur la biologie cutanée en particulier sur la morphologie et l'activité des mélanocytes. Les travaux de cette thèse ont porté sur les effets de la phénytoïne sur les mélanocytes humains afin de savoir si cette molécule peut être un traitement efficace pour le vitiligo. Dans un premier temps, nous avons évalué deux concepts : tout d'abord et pour la première fois, les effets in vitro des différentes concentrations de phénytoïne sur la morphologie et l'activité des mélanocytes humains, et parallèlement, nous avons mis en place la méthode du transfert de mélanosomes sur les mélanocytes et des kératinocytes humains. Dans un deuxième temps, nous avons procédé à l'évaluation in vivo de la forme topique à différentes concentrations à l'aide d'une étude in vivo sur des cochons d'Inde noirs. Notre travail constitue une étape clé dans la compréhension des mécanismes d'action de la phénytoïne sur les mélanocytes humains qui contribuerait à l'amélioration des pratiques cliniques et donc à la qualité de vie des patients souffrant de troubles pigmentaire. / Cutaneaous Biometrogy is a new vast spectrum of measuring methods wich provide the possibility to measure the différents parameteres of the skin even in the case of small changes. In the first part of this work, we studied various capabilities of these methods in order to correlates them with other clinical and histological data. These data encouraged us to discover more and more the skin pigmentation which is a little more complicated than the other parameters.So, on the second part, we concentrated more on cutaneaous biology particularily on the melanocytes morphology and activity.The work of this thesis focused on the effects of phenytoin on human melanocytes in order to know if this molecule can be eventually an available treatment for vitiligo.Fisrt, we evaluated two concepts : for the first time we evaluated the in vitro effects of the different concentrations of phenytoin on the morphology and activity of human melanocytes and, in parallel, we implemented the method of transfert of melanosomes on human melanocytes and keratinocytes.In a second step, the topical form of phenytoin at different concentrations was evaluated through an in vivo study on black ginea pigs.Our work is a key step on understanding the mechanisms of avtion of phenytoin on human melanocytes which would contribute to the improvement of clinical practices and therefore to the quality of life of patients suffering from depilatory disorders.

Biométrologie

Mélanocytes primares d'humains

Phénytoïne topique

Cochon d'inde noir

Repigmentation

Cutaneous biometrology

Primary human melanocytes

Topical phenytoin

Black guinea pigs

Repigmentation

616.5

Dissection of Zebrafish Adult Melanocyte Stem Cell Signaling During Regeneration

Frantz, William Tyler

26 May 2021

Tissue-resident stem cells are present in many adult organs, where they are important for organ homeostasis and repair in response to injury. However, the signals that activate these cells and the mechanisms governing how these cells self-renew or differentiate are highly context dependent and incompletely understood, particularly in non-hematopoietic tissues. In the skin, melanocyte stem cells (McSCs) are responsible for replenishing mature pigmented melanocytes. In mammals, these cells reside in the hair follicle bulge and bulb niches where they are activated during homeostatic hair follicle turnover and following melanocyte destruction, as occurs in vitiligo and other skin hypopigmentation disorders. Recently, we identified adult McSCs in the zebrafish. To elucidate mechanisms governing McSC self-renewal and differentiation fates we analyzed individual transcriptomes from thousands of melanocyte lineage cells during the regeneration process. We identified transcriptional signatures for McSCs, deciphered transcriptional changes and intermediate cell states during regeneration, and analyzed cell-cell signaling changes to discover mechanisms governing melanocyte regeneration. We identified KIT signaling via the RAS/MAPK pathway as a regulator of McSC direct differentiation. Analysis of the scRNAseq dataset also revealed a population of mitfa/aox5 co-expressing cells that divides following melanocyte destruction, likely corresponding to cells that undergo self-renewal. Our findings show how different subpopulations of mitfa-positive cells underlie regeneration and differentiation of at least one subpopulation requires reactivation of developmental KIT signaling to properly reconstitute the melanocyte stripe.

Melanocytes

Melanocyte Stem Cells

McSC

Zebrafish

Danio rerio

Melanoma

Vitiligo

Single cell transcriptomics

scRNAseq

KIT

c-KIT

kita

Cell Biology

Cellular and Molecular Physiology

Developmental Biology

The role of eicosanoids in the human skin's response to ultraviolet radiation.

Gledhill, Karl

January 2009

Erythema is a hallmark skin response to excessive ultraviolet radiation (UVR) and is associated with cutaneous inflammation. Both are mediated by inflammatory mediators including nitric oxide (NO), prostaglandin E2 (PGE2) and chemoattractants such as 12-hydroxyeicosatetraenoic acid (12-HETE) leading to vasodilation and increased leukocyte infiltration. The erythematous response is more pronounced in individuals with low basal melanin levels or who fail to respond to UVR with a robust up-regulation of melanogenesis. While melanin production is a key function of melanocytes, these cells can also produce NO and PGE2, and are located in close proximity to the dermal vasculature. It has been hypothesized that melanocytes with poor melanogenic capacity may participate in the inflammatory response to UVR. The aim of this project was to investigate the inflammatory response in the skin of individuals with either skin phototype (SPT) 1 or 4 to UVR. Sixteen normal healthy individuals were selected for study (8 SPT-1 & 8 SPT-4). Buttock skin was investigated by immunohistochemistry for leukocyte subtypes, eicosanoid producing enzymes and NO synthases under basal and UVR-stimulated conditions. In addition primary cultures of epidermal melanocytes (EM) were established from 16 individuals (8 SPT-1 & 8 SPT-4) and assessed for the presence of eicosanoid-producing enzymes, melanogenic enzymes and NO synthases, by immunocytochemistry, Polymerase Chain Reaction and Western Blotting and for the production of the main pro-inflammatory eicosanoid PGE2 by ELISA and Mass Spectrometry. Moreover, the fatty acid composition of cultured melanocytes was assessed by Gas Chromatography. Results showed that individuals with SPT-1 had significantly greater neutrophil infiltration into the epidermis than those with SPT-4 at 24 hrs post-UVR. Moreover, CD3+ lymphocyte infiltration into the dermis was significantly greater in individuals with SPT-4 than those with SPT-1 at 24 and 72 hrs post-UVR. NOS-1, NOS-3, 12-LOX and COX-2 expression were significantly increased in SPT-1 skin, while NOS-2 and 15-LOX were significantly increased in SPT-4 skin. As 12-LOX and COX-2 products are chemoattractive (for neutrophils) and pro-inflammatory respectively these data could explain the greater observed neutrophil infiltration in SPT-1. The 15-LOX product (15-HETE) is anti-inflammatory and may suggest that 15-LOX up-regulation in SPT-4 skin may aid resolution of the sunburn response, which in part may be mediated by CD3+ lymphocytes and a class-switch in eicosanoid production from COX to LOX products. Melanocyte primary cultures surprisingly showed that SPT was not correlated with melanin content or melanogenic enzyme expression/activity suggesting that all melanocytes in vitro contained the necessary cellular machinery to produce melanin. This finding may reflect also their equal treatment under these enriched culture conditions, which may or may not be available to these cells in situ. Moreover, all melanocytes expressed the necessary machinery (PLA2, COX-1, cPGES) to produce PGE2. However, only some cultures did so at baseline and in response to UVR, and this was not correlated with SPT. A positive correlation was found however between expression level of dopachrome tautomerase (DCT) and protection against PGE2 production in response to UVR, which may suggest a novel role for DCT unrelated to melanogenesis. In summary this research project has generated data that highlights differences between the skin of individuals with SPT-1 and those with SPT-4, and may provide evidence that the keratinocyte partner contributes significantly to the SPT-associated response. This research may also suggest DCT as a novel therapeutic target to protect EM from participation in the UVR-associated inflammatory response in skin. / Wellcome Trust

Erythema

Ultraviolet radiation (UVR)

Erythematous response

Melanocytes

Gas chromatography

Eicosanoids

Human skin response to UVR

Inflammation

Prostaglandin E2

Leukocyte

Melanin

Phototype

Dopachrome tautomerase

METABOLIC ACIDOSIS AND THE DIVERSE ROLES OF THE Cl/HCO₃ EXCHANGER (AE3) IN INTRACELLULAR pH HOMEOSTASIS

Salameh, Ahlam Ibrahim

January 2016

No description available.

Physiology

Nanoscience

Astrocytes

Cancer

Crosstalk

Dendritic Cells

Epilepsy

Hippocampus

Keratinocytes

Macrophages

Melanocytes

Mudullary raphe

Neurons

pH-regulation

Recovery Rate

Skeletal Muscles

Slc4

Novel roles for B-Raf in mitosis and cancer

Borysova, Meghan E. K.

January 2009

Dissertation (Ph.D.)--University of South Florida, 2009. / Title from PDF of title page. Document formatted into pages; contains 155 pages. Includes vita. Includes bibliographical references.

Estudo histomorfométrico, ultraestrutural e da expressão de Wnt1, WIF-1 e ASIP na pele com melasma em comparação com a pele sã perilesional e retroauricular

Lemos, Ana Cláudia Cavalcante Espósito

January 2017

Orientador: Hélio Amante Miot / Resumo: O melasma é hipermelanose crônica e adquirida decorrente de um complexo processo que envolve hipertrofia melanocítica e disfunção melanogênica. Acomete preferencialmente o sexo feminino e as lesões ocorrem nas áreas fotoexpostas, especialmente a face. Sua patogênese não é bem compreendida e os estudos clássicos avaliam apenas pele acometida e perilesional, mas pouco se sabe do comportamento da pele fotoprotegida, submetida aos mesmos fatores sistêmicos e genéticos. Neste estudo, objetivamos avaliar características histológicas, vias epidérmicas que influem na melanogênese (Wnt e ASIP) e características ultraestruturais da pele com melasma em comparação com a pele sã adjacente e retroauricular. Para a execução deste estudo transversal com controle intra-sujeito, foram coletadas três biópsias cutâneas (punch 3 mm) de onze mulheres com melasma facial. As áreas de coleta foram a pele com melasma, pele sã adjacente (distando no máximo 2 cm do limite da lesão) e pele retroauricular ipsilateral. Os fragmentos provenientes de dez participantes foram corados por hematoxilina-eosina, ácido periódico de Schiff, Fontana-Masson, picrosirius red, azul de toluidina e Verhöff; imunomarcados para CD34 e submetidos à imunofluorescência direta (IFD) de dupla marcação para proteínas Wnt1, WIF-1 e ASIP. Já os três fragmentos de uma das participantes foram processados para Microscopia Eletrônica de Transmissão (MET). Os dados obtidos foram comparados entre as topografias por modelo linear generali... (Resumo completo, clicar acesso eletrônico abaixo) / Mestre

Melanose.

Histologia.

Colágeno.

Melanose.

Melanócitos

Melanossomas

Histology

Sunlight

Collagen

Melanosis

Melanocytes

Melanosomes

Microscopia eletronica.

Radiação ultravioleta.

Luz solar

Microscopy, electron

Fluorescent antibody technique

Radiação ultravioleta.

Imunofluorescencia.

Fluorescent Antibody Technique, Direct

Estudo histomorfométrico, ultraestrutural e da expressão de Wnt1, WIF-1 e ASIP na pele com melasma em comparação com a pele sã perilesional e retroauricular / Histomorphometric and ultrastructural study, as well as evaluation of the expression of Wnt1, WIF-1 and ASIP on the skin of melasma compared to healthy skin adjacent and retroauricular

Lemos, Ana Cláudia Cavalcante Espósito [UNESP]

20 July 2017

Submitted by Ana Cláudia Cavalcante Espósito null (anaclaudiaesposito@gmail.com) on 2017-07-27T20:34:29Z No. of bitstreams: 1 Ana Cláudia mestrado para depositar.pdf: 2933638 bytes, checksum: 3c192abd021482675fa186f4c4bba9e4 (MD5) / Approved for entry into archive by LUIZA DE MENEZES ROMANETTO (luizamenezes@reitoria.unesp.br) on 2017-07-31T19:29:06Z (GMT) No. of bitstreams: 1 lemos_acce_me_bot.pdf: 2933638 bytes, checksum: 3c192abd021482675fa186f4c4bba9e4 (MD5) / Made available in DSpace on 2017-07-31T19:29:06Z (GMT). No. of bitstreams: 1 lemos_acce_me_bot.pdf: 2933638 bytes, checksum: 3c192abd021482675fa186f4c4bba9e4 (MD5) Previous issue date: 2017-07-20 / Fundo de Apoio à Dermatologia de São Paulo (FUNADERSP) / O melasma é hipermelanose crônica e adquirida decorrente de um complexo processo que envolve hipertrofia melanocítica e disfunção melanogênica. Acomete preferencialmente o sexo feminino e as lesões ocorrem nas áreas fotoexpostas, especialmente a face. Sua patogênese não é bem compreendida e os estudos clássicos avaliam apenas pele acometida e perilesional, mas pouco se sabe do comportamento da pele fotoprotegida, submetida aos mesmos fatores sistêmicos e genéticos. Neste estudo, objetivamos avaliar características histológicas, vias epidérmicas que influem na melanogênese (Wnt e ASIP) e características ultraestruturais da pele com melasma em comparação com a pele sã adjacente e retroauricular. Para a execução deste estudo transversal com controle intra-sujeito, foram coletadas três biópsias cutâneas (punch 3 mm) de onze mulheres com melasma facial. As áreas de coleta foram a pele com melasma, pele sã adjacente (distando no máximo 2 cm do limite da lesão) e pele retroauricular ipsilateral. Os fragmentos provenientes de dez participantes foram corados por hematoxilina-eosina, ácido periódico de Schiff, Fontana-Masson, picrosirius red, azul de toluidina e Verhöff; imunomarcados para CD34 e submetidos à imunofluorescência direta (IFD) de dupla marcação para proteínas Wnt1, WIF-1 e ASIP. Já os três fragmentos de uma das participantes foram processados para Microscopia Eletrônica de Transmissão (MET). Os dados obtidos foram comparados entre as topografias por modelo linear generalizado de efeitos mistos. As participantes eram fototipo III ou IV de Fitzpatrick, com idade média (desvio-padrão) de 42,9 (8,9) anos e apresentavam lesões há 16,7 (7,9) anos. Houve adelgaçamento da camada córnea na pele com melasma e na pele adjacente. Na pele com melasma houve maior compactação da córnea, maior pigmentação melânica epidérmica, maior heterogeneidade do colágeno, elastose solar, maior número de mastócitos, falhas da integridade da zona da membrana basal, melanócitos em pêndulo, bem como maior celularidade e vasos na derme superficial. IFD evidenciou maior intensidade de marcação de Wnt1 na pele com melasma em relação à pele adjacente e maior intensidade na pele retroauricular em relação à pele sã adjacente. Não houve diferença estatística significativa na intensidade de marcação de WIF-1 e ASIP entre as topografias. À MET, houve maior dano estrutural na lâmina lúcida no melasma, bem como maior número de melanossomas maduros e organelas citoplasmáticas nos melanócitos e queratinócitos basais. Tais resultados evidenciam que a pele com melasma apresenta, além da hipertrofia melanocítica, alterações na barreira epidérmica, na derme superior, zona de membrana basal e maior ativação da via Wnt, que diferem da pele fotoexposta adjacente e da retroauricular, configurando um fenótipo individualizado e não somente uma extensão do fotoenvelhecimento ou do envelhecimento intrínseco. / Melasma is a chronic and acquired hypermelanosis resulting from a complex process which involves melanocytic hypertrophy and melanogenic dysfunction. Melasma mainly affects females and lesions occur in the photoexposed areas, especially the face. Its pathogenesis is not well understood, and classical studies evaluate only the affected and perilesional skin, but little is known about the behavior of the non-sun-exposed skin, subjected to the same systemic and genetic factors. In this study, we aimed to evaluate histological features, epidermal pathways that influence melanogenesis (Wnt and ASIP) and ultrastructural characteristics of the skin with melasma in comparison to healthy adjacent and retroauricular skin. For the execution of this cross-sectional study with intrasubject control, three skin biopsies (punch 3 mm) were collected from eleven women with facial melasma. The areas of collection were the skin with melasma, adjacent healthy skin and retroauricular skin. Fragments from ten participants were stained with hematoxylin-eosin, periodic acid from Schiff, Fontana-Masson, picrosirius red, toluidine blue and Verhöff; immunomarked for CD34 and subjected to double-labeled direct immunofluorescence (DIF) for Wnt1, WIF-1 and ASIP proteins. The three fragments of one of the participants were processed for Transmission Electron Microscopy (TEM). The data obtained were compared between topographies by generalized linear model of mixed effects. Participants were Fitzpatrick's phototype III or IV; the mean age (standard deviation) was 42.9 (8.9) years and they had lesions for 16.7 (7.9) years. There was thinning of the corneal layer on the skin with melasma and adjacent skin. In the skin with melasma, there was more corneal compaction, greater epidermal melanic pigmentation, greater collagen heterogeneity, solar elastosis, more mast cells, defects of the basement membrane area, pendulum melanocytes, as well as greater cellularity and vessels in the superficial dermis. DIF showed a greater intensity of Wnt1 marking in the skin with melasma in relation to the adjacent skin, and greater intensity in the retroauricular skin in relation to the adjacent healthy skin. There was no significant statistical difference in the intensity of WIF-1 and ASIP marking between topographies. At TEM, there was more structural damage to the lamina lucida in melasma, as well as more mature melanosomes and cytoplasmic organelles in melanocytes and basal keratinocytes. These results show that melasma skin presents, in addition to melanocytic hypertrophy, alterations in the epidermal barrier, upper dermis, basement membrane zone and greater activation of the Wnt pathway, which differ from adjacent and retroauricular photoexposed skin, forming an individualized phenotype and not only an extension of photoaging or intrinsic aging.

Melasma

Microscopia eletrônica

Histologia

Luz solar

Raios ultravioletas

Colágeno

Melanose

Melanócitos

Melanossomas

Imunofluorescência

Microscopy, Electron

Histology

Sunlight

Ultraviolet rays

Collagen

Melanosis

Melanocytes

Melanosomes

Fluorescent antibody technique

Direct

Defining Mutation-Specific NRAS Functions that Drive Melanomagenesis

Murphy, Brandon M.

January 2021

No description available.

Biology

Biomedical Research

Cellular Biology

Molecular Biology

Oncology

cancer, biology

cell signaling

RAS

RAF

MAPK

mouse models

GEMM

molecular biology

cellular biology

cutaneous melanoma

melanoma

skin cancer

CRISPR-Cas9

melanocytes

fibroblasts

isolation

Stem cell factor/c-Kit signalling in normal and androgenetic alopecia hair follicles

Randall, Valerie A., Jenner, Tracey J., Hibberts, Nigel A., De Oliveira, Isabel O., Vafaee, Tayyebeh

January 2008

No / Androgens stimulate many hair follicles to alter hair colour and size via the hair growth cycle; in androgenetic alopecia tiny, pale hairs gradually replace large, pigmented ones. Since stem cell factor (SCF) is important in embryonic melanocyte migration and maintaining adult rodent pigmentation, we investigated SCF/c-Kit signalling in human hair follicles to determine whether this was altered in androgenetic alopecia. Quantitative immunohistochemistry detected three melanocyte-lineage markers and c-Kit in four focus areas: the epidermis, infundibulum, hair bulb (where pigment is formed) and mid-follicle outer root sheath (ORS). Colocalisation confirmed melanocyte c-Kit expression; cultured follicular melanocytes also exhibited c-Kit. Few ORS cells expressed differentiated melanocyte markers or c-Kit, but NKI/beteb antibody, which also recognises early melanocyte-lineage antigens, identified fourfold more cells, confirmed by colocalisation. Occasional similar bulbar cells were seen. Melanocyte distribution, concentration and c-Kit expression were unaltered in balding follicles. Androgenetic alopecia cultured dermal papilla cells secreted less SCF, measured by ELISA, than normal cells. This identifies three types of melanocyte-lineage cells in human follicles. The c-Kit expression by dendritic, pigmenting, bulbar melanocytes and rounded, differentiated, non-pigmenting ORS melanocytes implicate SCF in maintaining pigmentation and migration into regenerating hair bulbs. Less differentiated, c-Kit-independent cells in the mid-follicle ORS stem cell niche and occasionally in the bulb, presumably a local reserve for long scalp hair growth, implicate other factors in activating stem cells. Androgens appear to reduce alopecia hair colour by inhibiting dermal papilla SCF production, impeding bulbar melanocyte pigmentation. These results may facilitate new treatments for hair colour changes in hirsutism, alopecia or greying.

Adult

Alopecia

Metabolism

Androgens

Pharmacology

Cell lineage

Cells

Cultured

Female

Hair colour

Hair follicle

Cytology

Humans

Immunohistochemistry

Male

Melanins

Melanocytes

Chemistry

Middle aged

Proto-oncogene proteins c-kit

Signal transduction

Stem cell factor

REF 2014