Development of a virus‐based affinity ultrafiltration method for screening virus‐surface‐protein‐targeted compounds from complex matrixes: Herbal medicines as a case study

Author:

Li Zhongyuan1,Li Baohong2,Liu Miaomiao1,Chen Zinuo2,Li Ping3,Du Ruikun24ORCID,Su Ming5,Anirudhan Varada6ORCID,Achi Jazmin G.6ORCID,Tian Jingzhen14,Rong Lijun6,Cui Qinghua24

Affiliation:

1. College of Pharmacy Shandong University of Traditional Chinese Medicine Jinan China

2. Innovative Institute of Chinse Medicine and Pharmacy Shandong University of Traditional Chinese Medicine Jinan China

3. Key Laboratory of Chemical Biology (Ministry of Education), Department of Medicinal Chemistry, School of Pharmaceutical Sciences Shandong University Jinan China

4. Qingdao Academy of Chinese Medicinal Sciences Shandong University of Traditional Chinese Medicine Qingdao China

5. Shandong Academy of Chinese Medicine Jinan China

6. Department of Microbiology and Immunology, College of Medicine University of Illinois Chicago Chicago Illinois USA

Abstract

AbstractHerbal medicines (HMs) are one of the main sources for the development of lead antiviral compounds. However, due to the complex composition of HMs, the screening of active compounds within these is inefficient and requires a significant time investment. We report a novel and efficient virus‐based screening method for antiviral active compounds in HMs. This method involves the centrifugal ultrafiltration of viruses, known as the virus‐based affinity ultrafiltration method (VAUM). This method is suitable to identify virus specific active compounds from complex matrices such as HMs. The effectiveness of the VAUM was evaluated using influenza A virus (IAV) H1N1. Using this method, four compounds that bind to the surface protein of H1N1 were identified from dried fruits of Terminalia chebula (TC). Through competitive inhibition assays, the influenza surface protein, neuraminidase (NA), was identified as the target protein of these four TC‐derived compounds. Three compounds were identified by high performance liquid chromatography (HPLC) and liquid chromatography/mass spectrometry (LC/MS), and their anti‐H1N1 activities were verified by examining the cytopathic effect (CPE) and by performing a virus yield reduction assay. Further mechanistic studies demonstrated that these three compounds directly bind to NA and inhibit its activity. In summary, we describe here a VAUM that we designed, one that can be used to accurately screen antiviral active compounds in HMs and also help improve the efficiency of screening antiviral drugs found in natural products.

Publisher

Wiley

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