Selected article for: "genetic material and human virus"

Author: Singsuksawat, Ekapot; Onnome, Suppachoke; Posiri, Pratsaneeyaporn; Suphatrakul, Amporn; Srisuk, Nittaya; Nantachokchawapan, Rapirat; Praneechit, Hansa; Sae-kow, Chutimon; Chidpratum, Pala; Hongeng, Suradej; Avirutnan, Panisadee; Duangjinda, Thaneeya; Siridechadilok, Bunpote
Title: Potent programmable antiviral against dengue virus in primary human cells by Cas13b RNP with short spacer and delivery by virus-like particle
  • Cord-id: uk4kun8f
  • Document date: 2020_5_17
  • ID: uk4kun8f
    Snippet: With sequencing as a standard frontline protocol to identify emerging viruses such zika virus and SARS-CoV2, direct utilization of sequence data to program antivirals against the viruses could accelerate drug development to treat their infections. CRISPR-Cas effectors are promising candidates that could be programmed to inactivate viral genetic material based on sequence data but several challenges such as delivery and design of effective crRNA need to be addressed to realize practical use. Here
    Document: With sequencing as a standard frontline protocol to identify emerging viruses such zika virus and SARS-CoV2, direct utilization of sequence data to program antivirals against the viruses could accelerate drug development to treat their infections. CRISPR-Cas effectors are promising candidates that could be programmed to inactivate viral genetic material based on sequence data but several challenges such as delivery and design of effective crRNA need to be addressed to realize practical use. Here, we showed that virus-like particle (VLP) could deliver PspCas13b-crRNA ribonucleoprotein (RNP) in nanomolar range to efficiently suppress dengue virus infection in primary human target cells. Shortening spacer length could significantly enhance RNA-targeting efficiency of PspCas13b in mammalian cells compared to the natural length of 30 nucleotides without compromising multiplex targeting by a crRNA array. Our results demonstrate the potentials of applying PspCas13b RNP to suppress RNA virus infection, with implications in targeting host RNA as well.

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