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A Sendai Virus-Based Cytoplasmic RNA Vector as a Novel Platform for Long-Term Expression of MicroRNAs

Mol Ther Methods Clin Dev.. 2019; 
Sano M1, Nakasu A1, Ohtaka M1, Nakanishi M1.
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Gene Synthesis cDNAs encoding Hygr, human OCT4, SOX2, and KLF4 were synthesized by GenScript (Piscataway, NJ, USA). cDNAs encoding amiRNAs that included the complementary sequence for firefly luciferase,54 EGFP (NCBI: Pr008808666), or murine p53 (amip53#1: 5′-TGGGACAGCCAAGTCTGTTATG-3′, amip53#2: 5′-CGGGTGGAAGGAAATTTGTATC-3′) were prepared by PCR. These cDNAs were used to construct SeVdp genomic cDNAs as described previously.33 Preparation of vector packaging cells and the production of vectors were performed as described previously.33,55 Get A Quote

摘要

Cytoplasmic RNA virus-derived vectors have emerged as attractive vehicles for microRNA (miRNA) delivery as they possess no potential risk of chromosomal insertion. However, their relatively short-term expression limits their use in biological applications that require long-term miRNA manipulation, such as somatic cell reprogramming. Here, we show that a cytoplasmic RNA virus vector based on a replication-defective and persistent Sendai virus (SeVdp) serves as an effective platform for long-term production of miRNAs capable of inducing sequence-specific target suppression. The SeVdp vector was able to simultaneously deliver embryonic stem cell-enriched miRNAs, as well as multiple transcription factors, into fibr... More

关键词

RNA virus vector; Sendai virus; artificial miRNA; cell reprogramming; iPSCs; miRNA delivery