Dual-fluorescent reporter for live-cell imaging of the ER during DENV infection

Corliss, Lochlain; Holliday, Madeline; Lennemann, Nicholas J.

doi:10.3389/fcimb.2022.1042735

Cited by 2 publications

(1 citation statement)

References 61 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Previous research has shown that influenza A virus, foot and mouth disease viruses, Senecavirus A, West Nile virus and dengue virus have been engineered to carry a reporter gene for high throughput monoclonal antibody and antiviral assays [ 25 , 26 , 27 , 28 , 29 , 30 ]. Tagged EV-A71 and CV-A16 of the Enterovirus A are constructed by the same strategy to insert the GFP, nano luciferase, or gaussia luciferase gene between the 5′-UTR and the N-terminus of VP4, with the addition of a 2A protease cleavage site (ITTLG) at C-terminus of the 5′-UTR [ 13 , 14 , 15 , 16 , 17 ].…”

Section: Discussionmentioning

confidence: 99%

Reporter Coxsackievirus A5 Expressing iLOV Fluorescent Protein or Luciferase Used for Rapid Neutralizing Assay in Cells and Living Imaging in Mice

Jin,

Wang,

et al. 2023

Viruses

View full text Add to dashboard Cite

Coxsackievirus A5 (CV-A5) is a re-emerging enterovirus that causes hand, foot, and mouth disease in children under five years of age. CV-A5-M14-611 is a mouse-adapted strain that can infect orally and lead to the death of 14-day-old mice. Here, recombinants based on CV-A5-M14-611 were constructed carrying three reporter genes in different lengths. Smaller fluorescent marker proteins, light, oxygen, voltage sensing (iLOV), and nano luciferase (Nluc) were proven to be able to express efficiently in vitro. However, the recombinant with the largest insertion of the red fluorescence protein gene (DsRed) was not rescued. The construction strategy of reporter viruses was to insert the foreign genes between the C-terminus of VP1 and the N-terminus of 2A genes and to add a 2A protease cleavage domain at both ends of the insertions. The iLOV-tagged or Nluc-tagged recombinants, CV-A5-iLOV or CV-A5-Nluc, exhibited a high capacity for viral replication, genetic stability in cells and pathogenicity in mice. They were used to establish a rapid, inexpensive and convenient neutralizing antibody assay and greatly facilitated virus neutralizing antibody titration. Living imaging was performed on mice with CV-A5-Nluc, which exhibited specific bioluminescence in virus-disseminated organs, while fluorescence induced by CV-A5-iLOV was weakly detected. The reporter-gene-tagged CV-A5 can be used to study the infection and mechanisms of CV-A5 pathogenicity in a mouse model. They can also be used to establish rapid and sensitive assays for detecting neutralizing antibodies.

show abstract