Segmented GFP-like aptamer probes for functional imaging of viral genome trafficking.

Virus Res

Department of Chemistry, Indiana University, Bloomington, Indiana 47405, USA. Electronic address:

Published: December 2015

AI Article Synopsis

  • GFP-like RNA aptamers offer advantages for in vivo RNA imaging by enabling the co-packaging of viral genomes during virion assembly and trafficking.
  • The aptamer sequence can be split into two parts, allowing for self-assembly while maintaining the dye-binding pocket, resulting in virus-like particles that exhibit bright fluorescence and minimal bleaching, ideal for real-time studies.
  • In vivo experiments demonstrated the successful detection of aptamer-loaded virus-like particles in barley root cells, even amidst high levels of autofluorescence, showcasing their practical application for imaging.

Article Abstract

Recently developed GFP-like RNA aptamers harbor a few unique potential benefits for in vivo RNA imaging applications, including co-packaging of viral genomes. Here we examine them in the context of co-packaging of RNA strands during virion assembly and trafficking. The approach is applicable both in vitro and in vivo, thus bridging an existing methodological gap. We have found that splitting the aptamer sequence in the loop region into two separate parts allows for subsequent self-assembly into a functional unit, which preserves the dye-binding pocket. In presence of the dye, virus-like particles encapsulating segmented GFP-like aptamers provided bright fluorescence emission and showed negligible bleaching due to continuous chromophore exchange: two desirable characteristics for real-time in vivo single particle studies requiring a broader dynamic range than currently available. Proof-of-principle in vivo imaging experiments confirmed detectability of aptamer-loaded virus-like particles in barley root cells even in presence of significant autofluorescence background.

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Source
http://dx.doi.org/10.1016/j.virusres.2015.08.023DOI Listing

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