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Aldenine - clinical informationHuman skin is directly exposed to environmental aggression, mainly in the form of chemicals, air pollutants and UV irradiation. These factors generate reactive species (free radicals and others) responsible for extensive skin cell damage and aging.
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General principles on the working of Aldenine
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All the raw materials involved in the preparation of the product have been tested for the evaluation of primary skin irritation potential, sensitisation, ophthalmic irritation, oral and percutaneous toxicity. No signs of irritation or allergic reactions were observed.
Several tests were performed to prove the efficacy of both components, in both the RCS scavenger and Collagen III synthesis claims:
The graph shows how GHK is more effective than the endogenous scavenger carnosine (CAR) at capturing HNE in vitro.

Human Dermal Fibroblasts (HDF) were seeded at two different densities in 96-well culture plates and treated with Hydrolysed Vegetal Protein at different concentrations for 24 hours and 7 days. Collagen I and III were detected using an ELISA test with monoclonal antibodies. The increase in Collagen III can be seen even after 24 hours but a dose dependent result is obtained after 7 days.

Keratinocytes were photographed as: non-treated, treated with GHK, treated with HNE and treated with both. The pictures were repeated after irradiating the keratinocytes with a low UVB dose (50 mJ/cm2).
Note: this dose is enough to provoke erythema in people whose skin is phototype I to III (see table below)

The results presented in below show that irradiating keratinocytes with a low dose of UVB does not modify cellular morphology (top left photograph). GHK does not show a cytotoxic effect (top right photograph). In the bottom left photograph we can see that the cells cannot eliminate HNE since UVB depletes them of GSH, their natural scavenger. The picture shows clearly the deep morphological alterations due to HNE toxicity – non-confluent cells and vast areas of necrosis. The bottom right photograph proves that GHK is able to prevent damage by scavenging HNE and detoxifying the cell.

The following figures show the quenching activity of GHK versus HNE and ACR as a function of molar ratio, at 1 and 2 hours. It is clear that the results are dose-dependent and activity is continuing after 2 hours.
The potent RCS-scavenging activity of GHK is under patent by Lipotec SA.

It is known that some enzymes can suffer glycation in vivo. Among those enzymes we can find the Cu, Zn-Superoxide Dismutase (SOD). The SOD is an enzyme that converts superoxide radicals to hydrogen peroxide and oxygen. The incubation of SOD with glucose or other monosaccharides gives rise to glycation, which inactivates the enzyme. Some compounds can inhibit SOD glycation and, therefore, maintain its activity.
In this study, the inactivation of SOD by its reaction with fructose is used as a model of glycation. The effect of GHK as an inhibitor of glycation is evaluated. A method to assess the SOD activity by the inhibition of the transformation of xanthine to uric acid with the enzyme xanthine oxidase is used. With this reaction, the WST-1 (2-(4Iodophenyl)-3-(4-nitrophenyl)- 5-(2,4-disulfophenyl)-2H-tetrazolium, monosodium salt) is transformed to formazan, a compound which absorbs at 470nm. If SOD is added to this reaction, radical O2-. is captured and the formation of this coloured compound is avoided.
The results show there is and increase in the SOD activity, which means that GHK inhibits its glycation.

UVA radiation causes significant changes to skin cells, including DNA damage. DNA damage contributes to age-associated skin changes and DNA lesions caused by UVA radiation trigger photoaging of human skin.
Melanocytes were incubated with three different concentrations of ALDENINE® (1%, 2% and 4%) and cells were irradiated with UVA. Finally, induced DNA breaks were analyzed by the alkaline Comet assay.
Comet assay:

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