Re-structuring lentiviral vectors to express genomic RNA via cap-dependent translation
Author(s) -
John R. Counsell,
Guillaume De Brabandere,
Rajvinder Karda,
Marc T. Moore,
Antonio Greco,
Alysha Bray,
Juan Antinao Díaz,
Dany Perocheau,
Ulrike Mock,
Simon N. Waddington
Publication year - 2020
Publication title -
molecular therapy — methods and clinical development
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.285
H-Index - 32
ISSN - 2329-0501
DOI - 10.1016/j.omtm.2020.12.005
Subject(s) - biology , translation (biology) , rna , vector (molecular biology) , genome , provirus , viral vector , computational biology , transgene , gene , virology , genetics , messenger rna , recombinant dna
Lentiviral (LV) vectors based on human immunodeficiency virus type I (HIV-1) package two copies of their single-stranded RNA into vector particles. Normally, this RNA genome is reverse transcribed into a double-stranded DNA provirus that integrates into the cell genome, providing permanent gene transfer and long-term expression. Integration-deficient LV vectors have been developed to reduce the frequency of genomic integration and thereby limit their persistence in dividing cells. Here, we describe optimization of a reverse-transcriptase-deficient LV vector, which enables direct translation of LV RNA genomes upon cell entry, for transient expression of vector payloads as mRNA without a DNA intermediate. We have engineered a novel LV genome arrangement in which HIV-1 sequences are removed from the 5' end, to enable ribosomal entry from the 5' 7-methylguanylate cap for efficient translation of the vector payload. We have shown that this LV-mediated mRNA delivery platform provides transient transgene expression in vitro and in vivo . This has a potential application in gene and cell therapy scenarios requiring temporary payload expression in cells and tissues that can be targeted with pseudotyped LV vectors.
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