2014
DOI: 10.1534/g3.114.011197
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FluorescenceIn SituHybridization and Optical Mapping to Correct Scaffold Arrangement in the Tomato Genome

Abstract: The order and orientation (arrangement) of all 91 sequenced scaffolds in the 12 pseudomolecules of the recently published tomato (Solanum lycopersicum, 2n = 2x = 24) genome sequence were positioned based on marker order in a high-density linkage map. Here, we report the arrangement of these scaffolds determined by two independent physical methods, bacterial artificial chromosome–fluorescence in situ hybridization (BAC-FISH) and optical mapping. By localizing BACs at the ends of scaffolds to spreads of tomato s… Show more

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Cited by 86 publications
(91 citation statements)
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References 64 publications
(91 reference statements)
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“…In particular, root, leaf, flower, flower bud and six developmental stages of fruit (1, 2, 3 cm, mature green, breaker and mature red) tissues were considered. The gene expression level was defined on the basis of the iTAG mRNA loci (Shearer et al 2014) and was normalized by Reads Per Kilobases per Million (RPKM) for each tissue/ stage. Genes with expression level below 1 RPKM were considered as not expressed.…”
Section: Gene Expression Analysismentioning
confidence: 99%
See 1 more Smart Citation
“…In particular, root, leaf, flower, flower bud and six developmental stages of fruit (1, 2, 3 cm, mature green, breaker and mature red) tissues were considered. The gene expression level was defined on the basis of the iTAG mRNA loci (Shearer et al 2014) and was normalized by Reads Per Kilobases per Million (RPKM) for each tissue/ stage. Genes with expression level below 1 RPKM were considered as not expressed.…”
Section: Gene Expression Analysismentioning
confidence: 99%
“…However, addressing the role of the different pathways and the functionality of the different steps still remains a relevant issue. A major contribution to dissect these aspects can be provided by a suitable integration of data and resources today available for tomato (Chiusano et al 2008;Tomato Genome Consortium 2012;Shearer et al 2014;Bostan and Chiusano 2015). Driven by the recent increase of the ''omics'' data in tomato (Kusano and Fukushima 2013) the aim of this work is to gain insights into the AsA network architecture providing a complete gene survey for the biosynthetic, the recycling and the translocation pathways based on the current annotation of the tomato genome (iTAG2.40).…”
Section: Introductionmentioning
confidence: 99%
“…Scaffolds can contain errors in contig order (a 'translocation') or orientation (an 'inversion'). Examples of such errors can be found in the best available reference genomes for many species (Robert B. Norgren 2013;Shearer et al 2014;Tang et al 2014;Chen et al 2015;Davey et al 2016;Utsunomiya et al 2016;Schneider et al 2017;Korlach et al 2017). Consequently, inexpensive methods for identifying and correcting assembly errors are crucial for the generation of accurate assemblies (Salzberg and Yorke 2005;Phillippy, Schatz, and Pop 2008;Gnerre et al 2009;Tsai, Otto, and Berriman 2010;Salzberg et al 2012;Hunt et al 2013;Gurevich et al 2013;Bradnam et al 2013;Simão et al 2015;Fierst 2015;Muggli et al 2015;Yuan et al 2017;Harewood et al 2017).…”
mentioning
confidence: 99%
“…Miss-assembly and gaps in the sequence data are recurring problems in the assembly of any genome whether by whole genome shotgun approaches [58] [59] [60] or clone-by-clone approaches [61] [62]. Applications providing longer reads have fast become very popular for solving some of the issues associated with genome assemblies and platforms such as PacBio [55] and BioNano [51] show promise to improve the quality of shotgun assemblies.…”
Section: New Developmentsmentioning
confidence: 99%