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Cleavage of Stau2 by 3C protease promotes EV-A71 replication. | LitMetric

Cleavage of Stau2 by 3C protease promotes EV-A71 replication.

Virol J

Key Laboratory of Molecular Microbiology and Technology, Ministry of Education, College of Life Sciences, Nankai University, Tianjin, 300071, China.

Published: September 2024

AI Article Synopsis

  • Enterovirus A71 (EV-A71) primarily affects young children, causing illnesses like hand-foot-mouth disease and severe neurological complications; understanding its impact on the nervous system is important due to the viral protease 3C's role in this interaction.
  • This study confirmed that EV-A71 3C interacts with the host protein Staufen homolog 2 (Stau2), crucial for neuronal mRNA transport, and identified the specific cleavage site of Stau2 by the protease.
  • Findings indicate that Stau2 is vital for EV-A71 replication; while its overexpression boosts viral protein production, its depletion hinders it, highlighting Stau2 as a significant factor in the virus's life cycle.

Article Abstract

Background: Enterovirus A71 (EV-A71), as a neurotropic virus, mainly affects infants and young children under the age of 5. EV-A71 infection causes hand-foot-mouth disease and herpetic angina, and even life-threatening neurological complications. However, the molecular mechanism by which EV-A71 induces nervous system damage remains elusive. The viral protease 3C plays an important role during EV-A71 infection and is also a key intersection of virus-host interactions. Previously, we used yeast two-hybrid to screen out the host protein Double-stranded RNA-binding protein Staufen homolog 2 (Stau2), an important member involved in neuronal mRNA transport, potentially interacts with 3C.

Methods: We used coimmunoprecipitation (Co-IP) and immunofluorescence assay (IFA) to confirm that EV-A71 3C interacts with Stau2. By constructing the mutant of Stau2, we found the specific site where the 3C protease cleaves Stau2. Detection of VP1 protein using Western blotting characterized EV-A71 viral replication, and overexpression or knockdown of Stau2 exhibited effects on EV-A71 replication. The effect of different cleavage products on EV-A71 replication was demonstrated by constructing Stau2 truncates.

Results: In this study, we found that EV-A71 3C interacts with Stau2. Stau2 is cleaved by 3C at the Q507-G508 site. Overexpression of Stau2 promotes EV-A71 VP1 protein expression, whereas depletion of Stau2 by small interfering RNA inhibits EV-A71 replication. Stau2 is essential for EV-A71 replication, and the product of Stau2 cleavage by 3C, 508-570 aa, has activity that promotes EV-A71 replication. In addition, we found that mouse Stau2 is also cleaved by EV-A71 3C at the same site.

Conclusions: Our research provides an example for EV-A71-host interaction, enriching key targets of host factors that contribute to viral replication.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11401396PMC
http://dx.doi.org/10.1186/s12985-024-02489-6DOI Listing

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