2018
DOI: 10.1101/483693
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Direct RNA nanopore sequencing of full-length coronavirus genomes provides novel insights into structural variants and enables modification analysis

Abstract: Sequence analyses of RNA virus genomes remain challenging due to the exceptional genetic plasticity of these viruses. Because of high mutation and recombination rates, genome replication by viral RNA-dependent RNA polymerases leads to populations of closely related viruses, so-called 'quasispecies'. Standard (short-read) sequencing technologies are ill-suited to reconstruct large numbers of full-length haplotypes of (i) RNA virus genomes and (ii) subgenome-length (sg) RNAs comprised of noncontiguous genome reg… Show more

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Cited by 50 publications
(62 citation statements)
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References 70 publications
(58 reference statements)
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“…A similar observation showing a lower accuracy proximal to the 3' poly(A) tail has been observed previously due to the DNA adapter, which can partially explain poor accuracy at the 3' end [41,59]. agrees with what has been observed previously ( Figure 2) [44,45]. This is not surprising since the sequence adapter was ligated to the poly(A) tail on the 3' end and this is where sequencing began.…”
Section: Evaluation Of Minion Rna Sequencing For Generation Of Viral supporting
confidence: 91%
See 3 more Smart Citations
“…A similar observation showing a lower accuracy proximal to the 3' poly(A) tail has been observed previously due to the DNA adapter, which can partially explain poor accuracy at the 3' end [41,59]. agrees with what has been observed previously ( Figure 2) [44,45]. This is not surprising since the sequence adapter was ligated to the poly(A) tail on the 3' end and this is where sequencing began.…”
Section: Evaluation Of Minion Rna Sequencing For Generation Of Viral supporting
confidence: 91%
“…The U bases in the query sequence were adjusted to T automatically by the minimap program in order to map to the reference sequence which was DNA. The depth of coverage across the PRRSV genome was observed to be extremely uneven with higher coverage on the 3' end of the genome and gradually decreasing towards the 5' end, which agrees with what has been observed previously ( Figure 2) [44,45]. This is not surprising since the sequence adapter was ligated to the poly(A) tail on the 3' end and this is where sequencing began.…”
Section: Evaluation Of Minion Rna Sequencing For Generation Of Viral supporting
confidence: 89%
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“…As ONT-based native RNA-seq holds the capacity to sequence full-length transcripts, to identify RNA base modifications and to detect molecular heterogeneity in a transcriptome, the technology found widespread attention 16 . Recently, the technology was exploited to sequence viral RNA genomes 1720 to gain insights into viral and eukaryotic transcriptomes 19,2123 and to detect RNA isoforms in eukaryotes 24,25 . However, prokaryotic transcriptomes have not been characterized on the genome-wide level by native RNA-seq approaches so far as prokaryotic RNAs lack a poly(A) tail which is required to capture the RNA and feed it into the nanopore.…”
Section: Introductionmentioning
confidence: 99%