Minoxidil: mechanisms of action on hair growth

Messenger, A.G.; Rundegren, Jan

doi:10.1111/j.1365-2133.2004.05785.x

Cited by 506 publications

(405 citation statements)

References 62 publications

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“…However, the relative positive nuclear count frequencies for the different markers in other healthy human tissues are fully consistent with the majority of these zero counts being 'biological'. Whether low levels of markers could be reliably increased prestudy in order to make them more practicable, for example, through the use hair stimulants such as minoxidil (Messenger and Rundegren, 2004), is currently unknown. The final evaluation of the usefulness of any of these markers as study end points will depend on demonstrating PD activity on them within a future drug-intervention study.…”

Section: Discussionmentioning

confidence: 99%

Plucked human hair as a tissue in which to assess pharmacodynamic end points during drug development studies

et al. 2005

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We have demonstrated the feasibility of detecting and quantifying six cell-cycle-related nuclear markers (Ki67, pRb, p27, phosphop27 (phosphorylated p27), phospho-pRb (phosphorylated pRb), phospho-HH3 (phosphorylated histone H3)) in plucked human scalp and eyebrow hair. Estimates of the proportion of plucked hairs that are lost or damaged during processing plus the intra-and intersubject variability of each nuclear marker with these techniques are provided to inform sizing decisions for intervention studies with drugs potentially impacting on these markers in the future. (Moll, 1996;Gho et al, 2004); they are therefore potentially attractive as an easily accessible tissue in which to assess the pharmacodynamic (PD) effects of drugs that interfere with cell proliferation. Skin biopsies have already been used to similar ends during the development of a number of agents targeted against the epidermal growth factor receptor (Albanell et al, 2002;Malik et al, 2003;Salazar et al, 2004;Vanhoefer et al, 2004). Plucked hairs would offer certain advantages over skin biopsies for these purposes including improved tolerability, a greater potential for multiple time-point analyses and the possibility of a higher signal within hair follicles for certain key biomarkers compared to the cells of the epidermis (Albanell et al, 2002). We have developed a technique for quantifying cell-cycle-related proteins within the sheath cells of plucked human hair. MATERIALS AND METHODS Trial designIn all, 12 healthy Caucasian males, within the age range 18 -45 years, and with scalp hair greater than or equal to 5 mm in length, were recruited. Following thorough combing to remove any loose hairs, five suitable hairs with visible bulbs were plucked from each of the left eyebrow, right eyebrow and four different scalp sites using a pair of blunt-nosed forceps. Each set of five hairs was trimmed with scissors to a workable length (approximately 1 cm), retaining the bulb end of each hair, and then immersed in prelabelled 1.5 ml microcentrifuge tubes containing 1 ml 100% acetone at 41C. Plucked hairs without visible bulbs were discarded and not processed. Immunohistochemistry (IHC) and signal quantificationHair processing Following acetone fixation for 10 min, each hair was air-dried for 10 min and then placed, in batches of five from each sampling site, in 1 ml of 0.5 M, pH 7.6, Tris-buffered saline.Hair IHC In our hands, it was not possible to paraffin embed and then section the hairs for later staining without producing significant loss or damage of the fragile material; we therefore developed techniques based on staining intact hairs followed by rigid epoxy resin embedding and then sectioning.Briefly, a peroxidase block (5 min at room temperature), followed by a nonspecific protein block (30 min at room temperature), was employed on the intact hairs. A primary antibody, or buffer for negative controls, was then applied (antiKi67 at 1 : 100 for 1 h at room temperature, DAKO

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Section: Discussionmentioning

confidence: 99%

Plucked human hair as a tissue in which to assess pharmacodynamic end points during drug development studies

et al. 2005

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“…Finasteride and minoxidil are two well-known drugs for hair loss. 6,7 Finasteride is a synthetic 5-α-reductase inhibitor, and minoxidil is a vasodilator, both of which suppress male hormones and are used to treat alopecia. However, the use of two drugs should be limited due to strong side effects.…”

Section: Introductionmentioning

confidence: 99%

Visible-to-Near IR Quantum Dot–Based Hypermulticolor High-Content Screening of Herbal Medicines for the Efficacy Monitoring of Hair Growth Promotion and Hair Loss Inhibition

Kim

Lim

Lee³

et al. 2013

SLAS Discovery

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There is a growing interest in alopecia prevention strategies, as the number of alopecia patients is increasing. We examine the efficacy of herbal medicine for hair growth promotion/hair loss inhibition in two cell lines via Western blot and highcontent screening (HCS). Nine herbal extracts were obtained from three different herbal medicine mixtures using 3 different extraction methods. Five target proteins-IGF-1 (insulin-like growth factor-1), TGF-β2 (transforming growth factor-β2), VEGF (vascular endothelial growth factor), DKK-1 (Dickkopf-1), and Wnt5α-were observed for the assessment of hair growth promotion/hair loss inhibition efficacy. The efficacies of nine extracts were compared with minoxidil as control. Efficacy was defined as a rise in the expression levels of IGF-1, VEGF, and Wnt5α but a decrease in DKK-1 and TGF-β2. Intracellular concurrent imaging of these proteins was successfully achieved using HCS, employing visible-to-near infrared probing based on quantum-antibody conjugates and hypermulticolor imaging.

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“…현재까지 Minoxidil은 상피세포와 섬유아세포의 생장을 자극하거나 lysyl hydroxylase (LH)저해, 콜라겐 생성저해, prostaglandin E 2 (PGE 2 ) 합성을 자극하여 prostacyclin의 생 산저해 및 피부돌기 세포에 의한 VEGF (vascular endothelial growth factor)의 합성을 자극하는 것으로 알려졌다 [5]. 이 와 같이 세포기능에 다양한 영향을 미치고 있으나 어떤 표적 을 통하여 발모에 영향을 미치는지에 대한 연구는 부족한 실정이다.…”

Section: 서론unclassified

Structural Requirements of Minoxidil Analogs for Enhancing Lysyl Hydroxylase Inhibitory Activity

Myung¹,

Sung²,

Lee³

2012

KSBB Journal

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1) In order to explore structural features of minoxidil analogs with a view of enhancing lysyl hydroxylase (LH) inhibitory activity, molecular holographic QSAR (HQSAR) and CoMSIA (comparative molecular similarity indices analysis) were performed. The results from the atomic contributions with optimized the HQSAR 6-2 model indicated that, in case of pyrimidine-1-N-oxide substituent, C2 atom of pyrimidine ring and C'3-C'4 bond of 4-piperidinol group showed the highest impact on the inhibitory activity towards LH enzyme. It was also evident from the information of the optimized CoMSIA F5 model that the inhibitory activity mainly depended on the hydrophobic field contribution (36%) and the hydrogen bond (H-bond) field contribution (49.2%) of substrate molecule. Particularly, it is predicted that the functional groups which disfavor H-bond acceptors in large space around the piperidinol group and also the functional groups which favor the H-bond acceptors at C'4 (& C'5) atom

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Minoxidil: mechanisms of action on hair growth

Cited by 506 publications

References 62 publications

Plucked human hair as a tissue in which to assess pharmacodynamic end points during drug development studies

Plucked human hair as a tissue in which to assess pharmacodynamic end points during drug development studies

Visible-to-Near IR Quantum Dot–Based Hypermulticolor High-Content Screening of Herbal Medicines for the Efficacy Monitoring of Hair Growth Promotion and Hair Loss Inhibition

Structural Requirements of Minoxidil Analogs for Enhancing Lysyl Hydroxylase Inhibitory Activity

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