# Identification of Escherichia coli 166 isolate as an effective inhibitor of African swine fever virus replication

**Authors:** Jinya Zhang, Hongyu Cui, Zhenjiang Zhang, Wenqing Wang, Fengwei Jiang, Encheng Sun, Yuanmao Zhu, Fang Li, Zhigao Bu, Dongming Zhao

PMC · DOI: 10.1128/spectrum.03009-24 · 2025-02-26

## TL;DR

A specific strain of Escherichia coli, E. coli 166, was found to strongly inhibit the replication of African swine fever virus in pig cells, suggesting it could be a useful biological control agent.

## Contribution

The study identifies E. coli 166 as a novel, effective inhibitor of multiple African swine fever virus strains through indirect mechanisms.

## Key findings

- E. coli 166 inhibits replication of various African swine fever virus strains without direct cell contact.
- Both live and heat-inactivated E. coli 166 retain antiviral effects, suggesting metabolites or lysis products are responsible.
- Pretreatment with E. coli 166 modulates immune responses, upregulating NF-κB and downregulating CD163 in infected cells.

## Abstract

African swine fever is a lethal disease with mortality rates approaching 100% in both domestic pigs and wild boars. With no effective vaccines or treatments available, there is an urgent need for new biologics to combat the African swine fever virus (ASFV). In this study, we isolated bacteria from the intestinal contents of wild boar using culture-based methods and identified them through 16S ribosomal DNA (rDNA) sequencing. These isolates underwent high-throughput screening to evaluate their immunomodulatory effects on J774-Dual cells and their ability to inhibit ASFV replication in vitro. Among them, an Escherichia coli strain, designated as E. coli 166, exhibited strong inhibitory effects on various ASFV strains’ replication, including three genotype II strains: virulent strain HLJ/18, moderately virulent strain HLJ/HRB1/20, genetically modified low-virulent strain HLJ/18–6GD, and one genotype I low-virulent strain SD/DY-I/21. Notably, this inhibition did not require direct interaction between the bacteria and porcine alveolar macrophages (PAMs). Both live and heat-inactivated E. coli 166 demonstrated a strong inhibitory effect on ASFV replication. Genetic modification of E. coli 166 did not alter its inhibitory phenotype. Further analysis revealed that PAMs pretreated with E. coli 166 showed upregulation of NF-κB and downregulation of CD163 at different time points post-infection, whereas PAMs only infected with ASFV exhibited the opposite trend. These findings suggest that E. coli 166 holds promise as a biological agent for controlling ASFV infection, through indirect mechanisms involving bacterial metabolites or lysis products. Future studies should focus on identifying the specific components responsible for its antiviral effects.

The emergence of the African swine fever virus (ASFV) as a devastating pathogen in swine populations necessitates the development of novel strategies for its control. In this study, Escherichia coli strain 166 (E. coli 166) demonstrated a remarkable ability to inhibit the replication of multiple ASFV strains in porcine alveolar macrophages (PAMs), even without direct bacterial contact. Both live and heat-inactivated E. coli 166 retained this inhibitory effect, suggesting that secreted metabolites or lysis products may play a key role. Furthermore, pretreatment of PAMs with E. coli 166 resulted in upregulated NF-κB activity and downregulated expression of the ASFV entry receptor CD163, presenting an immune-modulatory mechanism distinct from PAMs solely infected with ASFV. These findings highlight the potential of E. coli 166 as a biological agent to combat ASFV, offering a promising alternative or complementary approach to traditional antiviral strategies.

## Linked entities

- **Genes:** NFKB1 (nuclear factor kappa B subunit 1) [NCBI Gene 4790], CD163 (CD163 molecule) [NCBI Gene 9332]
- **Diseases:** African swine fever (MONDO:0025377)
- **Species:** Escherichia coli (taxon 562)

## Full-text entities

- **Genes:** NFKB1 (nuclear factor kappa B subunit 1) [NCBI Gene 4790] {aka CVID12, EBP-1, KBF1, NF-kB, NF-kB1, NF-kappa-B1}, Cd163 (CD163 antigen) [NCBI Gene 93671] {aka CD163v2, CD163v3}, CD163 (CD163 molecule) [NCBI Gene 9332] {aka M130, MM130, SCARI1}, Nfkb1 (nuclear factor of kappa light polypeptide gene enhancer in B cells 1, p105) [NCBI Gene 18033] {aka NF-KB1, NF-kappaB, NF-kappaB1, p105, p50, p50/p105}
- **Species:** Allochromatium vinosum (species) [taxon 1049], Bacteria Latreille et al. 1825 (Bacteria stick insect, genus) [taxon 629395], African swine fever virus (no rank) [taxon 10497], Sus scrofa (pig, species) [taxon 9823], Suidae (boars, family) [taxon 9821], Escherichia coli (E. coli, species) [taxon 562]
- **Cell lines:** J774-Dual — Mus musculus (Mouse), Mouse reticulum cell sarcoma, Cancer cell line (CVCL_5I75), HLJ/18 — Homo sapiens (Human), Induced pluripotent stem cell (CVCL_8993)

## Figures

6 figures with captions in the complete paper: https://tomesphere.com/paper/PMC11960076/full.md

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Source: https://tomesphere.com/paper/PMC11960076