Rapid Generation of a Recombinant Genotype VIII Newcastle Disease Virus (NDV) Using Full-Length Synthetic cDNA

Rescue of (−)ssRNA viruses involves the sequential assembly and cloning of the full-length cDNA, which is often a challenging and time-consuming process. The objective of this study was to develop a novel method to rapidly clone the full-length cDNA of a very virulent NDV by only one assembly step....

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Veröffentlicht in:	Current microbiology 2021-04, Vol.78 (4), p.1458-1465
Hauptverfasser:	Murulitharan, Kavitha, Yusoff, Khatijah, Omar, Abdul Rahman, Peeters, Ben P. H., Molouki, Aidin
Format:	Artikel
Sprache:	eng
Schlagworte:	Animals Assembly Biomedical and Life Sciences Biotechnology Cloning Copy number DNA, Complementary - genetics Genomes Genotype Genotype & phenotype Genotypes Life Sciences Microbiology Mutation Newcastle disease Newcastle disease virus - genetics Pathogenicity Pathogens Plasmids Proteins RNA polymerase Sequences Transcription initiation Transfection Virulence Viruses
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container_title	Current microbiology
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creator	Murulitharan, Kavitha Yusoff, Khatijah Omar, Abdul Rahman Peeters, Ben P. H. Molouki, Aidin
description	Rescue of (−)ssRNA viruses involves the sequential assembly and cloning of the full-length cDNA, which is often a challenging and time-consuming process. The objective of this study was to develop a novel method to rapidly clone the full-length cDNA of a very virulent NDV by only one assembly step. A completely synthetic 15 kb cDNA of a Malaysian genotype VIII NDV known as strain AF2240-I with additional flanking Bsm BI sites was synthesised. However, to completely follow the rule-of-six, the additional G residues that are traditionally added after the T7 promoter transcription initiation site were not synthesised. The synthetic fragment was then cloned into low-copy number transcription vector pOLTV5-phiX between the T7 promoter and HDV Rz sequences through digestion with Bbs I. The construct was co-transfected with helper plasmids into BSRT7/5 cells. A recombinant NDV called rAF was successfully rescued using transfection supernatant harvested as early as 16 h post-transfection. Virus from each passage showed an intracerebral pathogenicity index (ICPI) and a mean death time (MDT) similar to the parent strain AF2240-I. Moreover, rAF possessed an introduced mutation which was maintained for several passages. The entire rescue using the one-step assembly procedure was completed within a few weeks, which is extremely fast compared to previously used methods.
doi_str_mv	10.1007/s00284-021-02421-z
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subjects	Animals Assembly Biomedical and Life Sciences Biotechnology Cloning Copy number DNA, Complementary - genetics Genomes Genotype Genotype & phenotype Genotypes Life Sciences Microbiology Mutation Newcastle disease Newcastle disease virus - genetics Pathogenicity Pathogens Plasmids Proteins RNA polymerase Sequences Transcription initiation Transfection Virulence Viruses
title	Rapid Generation of a Recombinant Genotype VIII Newcastle Disease Virus (NDV) Using Full-Length Synthetic cDNA
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