2016
DOI: 10.1073/pnas.1607532113
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Chromosome-level assembly ofArabidopsis thalianaLerreveals the extent of translocation and inversion polymorphisms

Abstract: Resequencing or reference-based assemblies reveal large parts of the small-scale sequence variation. However, they typically fail to separate such local variation into colinear and rearranged variation, because they usually do not recover the complement of large-scale rearrangements, including transpositions and inversions. Besides the availability of hundreds of genomes of diverse Arabidopsis thaliana accessions, there is so far only one full-length assembled genome: the reference sequence. We have assembled … Show more

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Cited by 193 publications
(295 citation statements)
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“…Interestingly, several sequences that flank the distal side of the two breakpoints are annotated as F‐box protein‐coding genes of the RNI‐like superfamily (https://www.arabidopsis.org), while the sequences at the proximal flank of both breakpoints are all Vandal5 transposon elements. Both the F‐box protein‐coding genes and the Vandal elements are present at the breakpoint positions in the L er genome (Zapata et al ., ), from which we can deduce that these elements are also in the knobless ancestor. The presence of Vandal5, a Mutator‐like (Mule) transposon, at the two breakpoints suggests that the inversion was created by the activity of the transposon.…”
Section: Resultsmentioning
confidence: 92%
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“…Interestingly, several sequences that flank the distal side of the two breakpoints are annotated as F‐box protein‐coding genes of the RNI‐like superfamily (https://www.arabidopsis.org), while the sequences at the proximal flank of both breakpoints are all Vandal5 transposon elements. Both the F‐box protein‐coding genes and the Vandal elements are present at the breakpoint positions in the L er genome (Zapata et al ., ), from which we can deduce that these elements are also in the knobless ancestor. The presence of Vandal5, a Mutator‐like (Mule) transposon, at the two breakpoints suggests that the inversion was created by the activity of the transposon.…”
Section: Resultsmentioning
confidence: 92%
“…The L er fragment thus provided us the precise map positions of the distal and proximal breakpoints at 1 612 609 bp and 2 782 618 bp, respectively. The de novo assembly of the L er ‐0 sequence confirmed the two breakpoint positions (Zapata et al ., ). The entire inversion spans 1.17 Mb and contains 145 protein‐coding genes.…”
Section: Resultsmentioning
confidence: 97%
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“…Recently, several high-quality genome assemblies have been published using one or both technologies [9][10][11][12][13][14] . The use of long-read sequencing technologies may also tackle potential assembly issues that are related to the presence of highly similar sequences resulting from whole-genome duplication events that frequently occurred in angiosperm genomes 15 .…”
mentioning
confidence: 99%
“…Indeed, de novo sequencing of a BG‐5 fosmid library revealed a large transposition at a location 4 Mb upstream that moved a fragment of size 70 kb from within the mapping interval (22.52–22.59 Mb). The same transposition was found in other A. thaliana accessions (Wijnker et al ., ; Zapata et al ., ) which did not cause the same hybrid phenotype when crossed to Kro‐0, ruling out any role for the transposed region in the phenotype. Nevertheless, excluding the transposition reduced the final mapping interval to 22.07–22.52 Mb (450 kb).…”
Section: Resultsmentioning
confidence: 94%