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China Surfactant Detergent & Cosmetics ›› 2023, Vol. 53 ›› Issue (11): 1280-1284.doi: 10.3969/j.issn.2097-2806.2023.11.006

• Development and application • Previous Articles     Next Articles

The establishment and application of an in vitro evaluation system for 5α-reductase inhibitors

Pan Jifei1,3,4,Wang Xiaona2,Guo Haijiao2,Yang Suzhen2,Chen Jianying1,3,4,*()   

  1. 1. Shandong Academy of Pharmaceutical Sciences, Jinan, Shandong 250101, China
    2. Shandong Freda Biotech Co., Ltd., Jinan, Shandong 250101, China
    3. Shandong Provincial Engineering Research Center for Skin and Mucosal Drug Delivery, Shandong Academy of Pharmaceutical Sciences, Jinan, Shandong 250101, China
    4. Shandong Engineering Research Center of Novel Sustained and Controlled Release Formulations and Targeted Drug Delivery Systems, Shandong Academy of Pharmaceutical Sciences, Jinan, Shandong 250101, China
  • Received:2023-05-30 Revised:2023-10-24 Online:2023-11-22 Published:2023-11-21
  • Contact: *Tel.: +86-15066696396, E-mail: chenjy_@hotmail.com.

Abstract:

5α-reductase (5AR) is a microsomal enzyme that relies on reducing coenzyme Ⅱ (NADPH) as a hydrogen donor to irreversibly convert testosterone to dihydrotestosterone (DHT). There are three isoenzymes in the alpha-reductase family, namely Ⅰ (5AR1), Ⅱ (5AR2) and Ⅲ (5AR3). Two distinct isozymes are found in mouse, rat, monkey, and human: 5AR1 and 5AR2. In human, 5AR1 is predominant in the sebaceous glands of most regions of skin, including scalp, and liver. 5AR1 is responsible for approximately one-third of the circulating DHT. 5AR2 isozyme is primarily found in prostate, seminal vesicles, epididymites, hair follicles as well as liver, and is responsible for two-thirds of the circulating DHT. 5AR1 in sebaceous gland cells plays a certain role in local androgen metabolism, stimulation of excessive sebum secretion and the occurrence of acne. The high level of DHT is easy to cause acne and other skin problems. According to the above reaction principles, an in vitro model was established to screen 5AR inhibitors. The reaction system was divided into four groups: Blank control, Negative control, Positive control and Sample group. 5AR was prepared from the liver of SD rats. The content of testosterone was determined by HPLC method using Dutastamide, which had strong inhibition on both 5AR1 and 5AR2, as the positive control. Specificity test shows that other components have no interference on the determination of testosterone, and the method has good specificity. Correlation coefficient r is 0.999 7, testosterone has a good linear relationship in the range of 0.059-9.860 μg/mL, and the limit of quantitation (S/N≥10) is 0.059 μg/mL. RSDs of the precision test are 0.3%, and the precision is good. RSDs of the repeatability test are 0.7%, indicating that the method has good repeatability. Several samples were screened using this screening model, and several samples such as zinc hyaluronate shows strong inhibition of 5AR. This model can effectively screen 5AR inhibitors, and provide reference for the development of oil-control, anti-acne and other products. Compared with other existing androgen antagonists, 5AR inhibitor selectively blocks DHT synthesis while not affecting the normal level and physiological function of testosterone, and inhibits 5AR as an important method for the treatment of benign prostatic hyperplasia, male alopecia and other androgen-dependent diseases. With the inhibition of 5AR activity as the target, steroid and non-steroid 5AR inhibitors from various sources are becoming a hot spot in drug development.

Key words: 5α-reductase, inhibitors, HPLC

CLC Number: 

  • TQ658