In vitro susceptibility of human Blastocystis subtypes to simeprevir

Shereen F Mossallam; Salwa A T El-Mansoury; Mona M Tolba; Asmaa A Kohla; Safaa I Khedr

doi:10.1016/j.sjbs.2021.01.050

In vitro susceptibility of human Blastocystis subtypes to simeprevir

Saudi J Biol Sci. 2021 Apr;28(4):2491-2501. doi: 10.1016/j.sjbs.2021.01.050. Epub 2021 Feb 2.

Authors

Shereen F Mossallam¹, Salwa A T El-Mansoury¹, Mona M Tolba², Asmaa A Kohla¹, Safaa I Khedr¹

Affiliations

¹ Department of Medical Parasitology, Faculty of Medicine, Alexandria University, Alexandria, Egypt.
² Department of Parasitology, Medical Research Institute, Alexandria University, Alexandria, Egypt.

Abstract

Introduction and aim: Blastocystis is a common enteric parasite, having a worldwide distribution. Many antimicrobial agents are effective against it, yet side effects and drug resistance have been reported. Thus, ongoing trials are being conducted for exploring anti-Blastocystis alternatives. Proteases are attractive anti-protozoal drug targets, having documented roles in Blastocystis. Serine proteases are present in both hepatitis C virus and Blastocystis. Since drug repositioning is quite trendy, the in vitro efficacy of simeprevir (SMV), an anti-hepatitis serine protease inhibitor, against Blastocystis was investigated in the current study.

Methods: Stool samples were collected from patients, Alexandria, Egypt. Concentrated stools were screened using direct smears, trichrome, and modified Ziehl-Neelsen stains to exclude parasitic co-infections. Positive stool isolates were cultivated, molecularly subtyped for assessing the efficacy of three SMV doses (100,150, and 200 μg/ml) along 72 hours (h), on the most common subtype, through monitoring parasite growth, viability, re-culture, and also via ultrastructure verification. The most efficient dose and duration were later tested on other subtypes.

Results: Results revealed that Blastocystis was detected in 54.17% of examined samples. Molecularly, ST3 predominated (62%), followed by ST1 (8.6%) and ST2 (3.4%). Ascending concentrations of SMV progressively inhibited growth, viability, and re-culture of treated Blastocystis, with a non-statistically significant difference when compared to the therapeutic control metronidazole (MTZ). The most efficient dose and duration against ST3 was 150 µg/ml for 72 h. This dose inhibited the growth of ST3, ST1, and ST2 with percentages of 95.19%, 94.83%, and 94.74%, successively and viability with percentages of 98.30%, 98.09%, and 97.96%, successively. This dose abolished Blastocystis upon re-culturing. Ultra-structurally, SMV induced rupture of Blastocystis cell membrane leading to necrotic death, versus the reported apoptotic death caused by MTZ. In conclusion, 150 µg/ml SMV for 72 h proved its efficacy against ST1, ST2, and ST3 Blastocystis, thus sparing the need for pre-treatment molecular subtyping in developing countries.

Keywords: Blastocystis subtypes; CV, central vacuole; DMSO, Dimethyl Sulfoxide; IBS, irritable bowel syndrome; In vitro; MLO, Mitochondrion-like organelle; MTZ, Metronidazole; PCR, Polymerase chain reaction; Re-culture; SEM, Scanning electron microscopy; SMV, Simeprevir; ST, subtypes; Simeprevir; TEM, Transmission electron microscopy; Ultrastructure; Viability.