Mechanism of Selective Qβ Bacteriophage Inactivation under the Presence of E. Coli Using Ground Rh-Doped SrTiO3 Photocatalyst

Author:

Usuki Sho1,Machida Shingo2ORCID,Katsumata Ken-ichi2ORCID,Ogawa Makoto34,Latthe Sanjay S.5,Liu Shanhu6,Yamatoya Kenji7ORCID,Nakata Kazuya1ORCID

Affiliation:

1. Graduate School of Bio-Applications and Systems Engineering, Tokyo University of Agriculture and Technology, 2-24-16 Naka-cho, Koganei, Tokyo 184-0012, Japan

2. Department of Material Science and Technology, Faculty of Advanced Engineering, Tokyo University of Science, 6-3-1 Niijuku, Katsushika-ku, Tokyo 125-8585, Japan

3. School of Energy Science and Engineering, Vidyasirimedhi Institute of Science and Technology, 555 Moo 1 Tumbol Payupnai, Amphoe Wangchan, Rayong 21210, Thailand

4. Japan Advanced Institute of Science & Technology, 1-1 Asahidai, Nomi 923-1292, Ishikawa, Japan

5. Vivekanand College, C.S. No 2130 E Ward, Tarabai Park, Kolhapur 416 003, Maharashtra, India

6. Henan Key Laboratory of Polyoxometalate Chemistry, Henan Joint International Research Laboratory of Environmental Pollution Control Materials, College of Chemistry and Chemical Engineering, Henan University, Kaifeng 475004, China

7. Laboratory of Genomic Function Engineering, Department of Life Sciences, School of Agriculture, Meiji University, 1-1-1 Higashimita, Tama-Ward, Kawasaki 214-8571, Kanagawa, Japan

Abstract

Photocatalysts have recently attracted attention for removing infectious-disease-causing bacteria and viruses. Among such photocatalysts, ground Rh-doped SrTiO3 (“g-STO:Rh”) has been found to have biospecificity that reduces the Qβ phage infectivity under conditions that did not decrease the E. coli survival rate. Elucidating the mechanism of selective antiphage activation is important for developing photocatalysts that act effectively against specific microorganisms. In this study, SDS-PAGE and quantitative PCR showed that a g-STO:Rh-treated Qβ phage preferentially inactivated the A2 protein involved in attachment to host cells. The analysis of the photocatalyst-treated ovalbumin using g-STO:Rh indicated that the protein’s isoelectric point significantly influenced the initial interaction with g-STO:Rh. However, once the protein is absorbed, it was decomposed without the release of intermediates. Furthermore, an inactivation assay for four different phages by photocatalyst treatment using g-STO:Rh revealed that phages with positively charged proteins are highly susceptible to inactivation, and the accessibility of critical components to g-STO:Rh influences susceptibility. We conclude that the selective antiphage activation of g-STO:Rh depends on the adsorption efficiency of the protein and g-STO:Rh.

Funder

New Energy and Industrial Technology Development Organization

Publisher

MDPI AG

Subject

Physical and Theoretical Chemistry,Catalysis,General Environmental Science

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