Journal
PLANT JOURNAL
Volume 57, Issue 4, Pages 758-770Publisher
WILEY
DOI: 10.1111/j.1365-313X.2008.03720.x
Keywords
ribonucleic acid; live-cell imaging; virus; replication; Pumilio; bimolecular fluorescence complementation
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Funding
- European Commission
- Darwin Trust
- BBSRC [BB/E001564/1, BB/D010462/1] Funding Source: UKRI
- Biotechnology and Biological Sciences Research Council [BB/D010462/1, BB/E001564/1] Funding Source: researchfish
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We describe a method for localizing plant viral RNAs in vivo using Pumilio, an RNA-binding protein, coupled to bimolecular fluorescence complementation (BiFC). Two Pumilio homology domain (PUMHD) polypeptides, fused to either the N- or C-terminal halves of split mCitrine, were engineered to recognize two closely adjacent eight-nucleotide sequences in the genomic RNA of tobacco mosaic virus (TMV). Binding of the PUMHDs to their target sites brought the split mCitrine halves into close proximity, allowing BiFC to occur and revealing the localization of viral RNA within infected cells. The bulk of the RNA was sequestered in characteristic inclusion bodies known as viral replication complexes (VRCs), with a second population of RNA localized in discrete particles distributed throughout the peripheral cytoplasm. Transfer of the TMV Pumilio recognition sequences into the genome of potato virus X (PVX) allowed the PVX RNA to be localized. Unlike TMV, the PVX RNA was concentrated in distinctive 'whorls' within the VRC. Optical sectioning of the PVX VRCs revealed that one of the viral movement proteins was localized to the centres of the RNA whorls, demonstrating significant partitioning of viral RNA and proteins within the VRC. The utility of Pumilio as a fluorescence-based reporter for viral RNA is discussed.
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