Zebrafish C-reactive protein isoforms inhibit SVCV replication by blocking autophagy through interactions with cell membrane cholesterol

Melissa Bello-Perez,Luis Perez,Beatriz Novoa,Alberto Falco,Julio Coll,Patricia Pereiro

doi:10.1038/s41598-020-57501-0

Abstract

In the present work, the mechanisms involved in the recently reported antiviral activity of zebrafish C-reactive protein-like protein (CRP1-7) against the spring viraemia of carp rhabdovirus (SVCV) in fish are explored. The results neither indicate blocking of the attachment or the binding step of the viral replication cycle nor suggest the direct inhibition of G protein fusion activity or the stimulation of the host’s interferon system. However, an antiviral state in the host is induced. Further results showed that the antiviral protection conferred by CRP1-7 was mainly due to the inhibition of autophagic processes. Thus, given the high affinity of CRPs for cholesterol and the recently described influence of the cholesterol balance in lipid rafts on autophagy, both methyl-β-cyclodextrin (a cholesterol-complexing agent) and 25-hydroxycholesterol (a cholesterol molecule with antiviral properties) were used to further describe CRP activity. All the tested compounds exerted antiviral activity by affecting autophagy in a similar manner. Further assays indicate that CRP reduces autophagy activity by initially disturbing the cholesterol ratios in the host cellular membranes, which in turn negatively affects the intracellular regulation of reactive oxygen species (ROS) and increases lysosomal pH as a consequence. Ultimately, here we propose that such pH changes exert an inhibitory direct effect on SVCV replication by disrupting the pH-dependent membrane-fusogenic ability of the viral glycoprotein G, which allows the release of the virus from endosomes into cytoplasm during its entry phase.

Highlights

In the present work, the mechanisms involved in the recently reported antiviral activity of zebrafish C-reactive protein-like protein (CRP1-7) against the spring viraemia of carp rhabdovirus (SVCV) in fish are explored
Our previous studies showed that the treatment with the supernatant from epithelioma papulosum cyprinid (EPC) cells that had been transfected with zebrafish CRP1-7 inhibited SVCV infection in vitro[42,47]; whether such anti-viral activity might be due to the interaction of CRP1-7 with viral particles remains to be demonstrated
When either EPC cells (Fig. 1A) or SVCV (Fig. 1B) were treated with CRP1-7 prior to the viral adsorption stage, similar, significant inhibition of SVCV replication activities were observed for all CRPs (CRP2-6 inhibition was in the range of 47.1-76.2%), except for CRP1 and CRP7

Summary

Introduction

The mechanisms involved in the recently reported antiviral activity of zebrafish C-reactive protein-like protein (CRP1-7) against the spring viraemia of carp rhabdovirus (SVCV) in fish are explored. Phosphorylcholine works as a pathogen-associated molecular pattern (PAMP)[10,18,19,20], and as a danger-associated molecular pattern (DAMP)[18,21,22,23,24] This phosphorylcholine-binding site of the soluble CRP is involved in interactions with, for instance, oxidized low-density lipoprotein (LDL)[21], nuclear materials (such as chromatin, histones, small nuclear ribonucleoproteins)[25,26], and other compounds that may not contain phosphorylcholine but are abundant in bacteria[27], fungi[28,29] and parasites[30,31]

Methods

Results

Conclusion