Skin care research: Topical delivery of retinyl ascorbate co-drug. 5. In vitro degradation studies.

Intelligent anti-aging skin care based on independent research

Lose wrinkles, keep your bank account!

Skin Care 101

Skin Care Basics

Skin Protection

Skin Biology

Biology of Aging

Ingredient Guide

Skin & Nutrition

Skin Conditions

Anti-Aging Treatments

Topical Actives

Wrinkle Fillers

Noninvasive

Invasive

Skin Care Smarts

Smart Choices

Best Practices

Find Good Skin Doc

Quick Tips

Freebie Finder

Reviews & Research

Product Reviews

Provider Reviews

Skin Care Research

Clinical Trials

How-To Infopacks

Skin Rejuvenation

DIY Skin Care

Skin & Nutrition

Eye Skin Care

Longevity In a Pill

Community & Misc

Forums

Polls & Surveys

News and Updates

Search

-- advertisements --

You are here: Skin Care Research >

Topical delivery of retinyl ascorbate co-drug. 5. In vitro degradation studies.

Author: Abdulmajed K, McGuigan C, Heard CM

Author affiliation: Welsh School of Pharmacy, Cardiff University, Cardiff, UK.

Publication date & source: 2006, Skin Pharmacol Physiol., 19(5):248-58. Epub 2006 Jun 16.

Chemical and enzymatic hydrolysis of the co-drug of retinoic acid (vitamin A) and ascorbic acid (vitamin C) - retinyl ascorbate (RA-AsA)--have been studied. Firstly, the amount of protein and ester hydrolysis activity was determined in crude cellular extracts from freshly excised porcine ear skin (<3 h) and stored porcine ear skin (frozen >6 months) using ethyl butyrate as model substrate. The stability of RA-AsA was then determined in the crude cell extracts with and without additional antioxidants. Lastly, the enzymatic hydrolysis of RA-AsA and retinyl-2-carboxy-2-hydroxy-ethanoate were determined by incubating with porcine liver esterase - retinol palmitate and ascorbyl palmitate were included for comparison. Freshly excised skin contained higher amounts of active proteins than previously frozen skin. RA-AsA underwent hydrolytic reduction causing the AsA moiety to disintegrate due to the presence of free radicals in the media. An intermediate was produced that seemed to be cleaved by enzymes. Addition of ascorbic acid, as antioxidant, to the media of crude protein extracts decelerated the hydrolysis rate. This was supported when RA-AsA and retinyl-2-carboxy-2-hydroxy-ethanoate were incubated separately with pure esterase. There was approximately 5-fold more soluble protein per ml of cytosol in the fresh skin compared to the stored skin. Therefore, the amount of protein present within approximately 1.5 cm(2) of skin (average diffusion area in the Franz cells used in our skin penetration studies) was 0.06 mg cm(-2) and 0.01 mg cm(-2) for fresh and stored extracts, respectively.

Indexes of Skin Care Research Abstracts
by Subject Category	Most Recent

-- advertisements --