A Comparative Genomics Strategy for Targeted Discovery of Single-Nucleotide Polymorphisms and Conserved-Noncoding Sequences in Orphan Crops

Feltus, F. Alex; Singh, Harvinder; Lohithaswa, H. C.; Schulze, Stefan; Silva, T.D.; Paterson, Andrew H.

doi:10.1104/pp.105.074203

Cited by 89 publications

(74 citation statements)

References 35 publications

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“…The development of SSRs based on EST sequences is a fast, efficient, and economic option [35][36][37][38]. In addition, a new generation of marker system termed single-strand conformational polymorphism-single nucleotide polymorphism (SSCP-SNP) has been developed in pearl millet to take advantage of the SSCP technique and the large number of SNPs in the nonexpressed intron regions of genes [39], which are also the target of the conserved intron-spanning primer (CISP) markers [40]. SNP markers provide an inexhaustible source of polymorphic markers for use in high-resolution genetic mapping and are the most abundant type of molecular genetic markers in the genome.…”

Section: Introductionmentioning

confidence: 99%

Construction of Genetic Linkage Map and QTL Analysis of Sink-Size Traits in Pearl Millet (Pennisetum glaucum)

Vengadessan¹,

Rai

Bapu

et al. 2013

ISRN Genetics

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A linkage map, primarily based on SSCP-SNP markers, was constructed using 188 F 2:3 mapping population progenies produced from a cross between two pearl millet inbred lines having diverse parentage. The skeleton linkage map covered 1019 cM and it comprised of 44 markers distributed across the seven linkage groups. Average adjacent-marker intervals ranged from 14 cM on LG1 to 38 cM on LG6, with an overall mean of 23 cM. Using the F 2 linkage map and phenotypic data from the F 2 and F 2:3 generations of the mapping population, a total of 18 putative QTLs were detected for the three sink-size components. Eight QTLs explained 42.7% of observed phenotypic variation for panicle length using the F 2:3 data set. For panicle diameter, 5 QTLs explained 45.8% of observed phenotypic variation. Similarly for grain size, 5 QTLs explained 29.6% of phenotypic variation. Genomic regions associated with panicle length, panicle diameter, and grain size were comapped on LG6 between Xpsms88 and Xpsms2270, indicating the existence of a gene or gene cluster. The QTLs for panicle length on LG2 and LG6 (LOD > 3 in both F 2 and F 2:3 data sets), for panicle diameter on LG2 and LG3 (LOD > 14 in the F 2:3 data set), and for grain size on LG3 and LG6 (LOD > 3 in both F 2 and F 2:3 data sets) were identified as promising candidates for validation prior to possible application in marker-assisted breeding.

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Section: Introductionmentioning

confidence: 99%

Construction of Genetic Linkage Map and QTL Analysis of Sink-Size Traits in Pearl Millet (Pennisetum glaucum)

Vengadessan¹,

Rai

Bapu

et al. 2013

ISRN Genetics

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“…In pearl millet, although marker aided-selection (MAS) has not been practiced yet in breeding for Striga resistance, there have been extensive efforts towards development of DNA-based markers including simple sequence repeat (SSR) Budak et al, 2003;Mariac et al, 2006;Qi et al 2001Qi et al , 2004Senthilvel et al, 2004Senthilvel et al, , 2008Jia et al, 2007;Yadav et al, 2007Yadav et al, , 2008Rajaram et al, 2013), diversity array technology (DArT) (Mace et al, 2008(Mace et al, , 2009Supriya et al, 2011) and single nucleotide polymorphism (SNP) (Bertin et al, 2005;Feltus et al, 2006;Kountche, 2013;Moumouni et al, 2015). In most of these studies, a number of genetic maps have been constructed using different crosses, mostly with the aim of mapping specific traits.…”

Section: Marker-assisted Selectionmentioning

confidence: 99%

Striga

Kountche

Al‐Babili

Haussmann

2016

Biotic Stress Resistance in Millets

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“…In case of well-characterized species, exonintron boundaries can be defined using tools like FEGNESH, etc. and subsequently primer pairs can be designed using the flanking exonic sequence of an intron to amplify intronic region (Feltus et al 2006). By using the genome sequence data of Medicago and Lotus and EST data of soybean and Medicago, >3,000 primer pairs targeting intronic regions have been developed in the laboratory of Doug Cook at UC-Davis, USA (DR Cook, personal communication) to develop gene-based conserved orthologous sequence (COS) markers in legume species.…”

Section: Intron Targeted Marker Development By Using Comparative Genomentioning

confidence: 99%

“…In this way, intronic sequence can be identified and exonic sequence of the ESTs are used to design the primer pairs to amplify the intronic region. Based on this concept, after aligning the ESTs of sorghum, pearl millet, Allium and Musa with rice genome, >3,600 primer pairs, called conserved intron spanning primers (CISPs) have been developed for monocot species (Feltus et al 2006;Lohithaswa et al 2007; http://www.plantgenome.uga.edu/CISP/). Following the similar approach, a larger number of gene-based markers have been developed and used for diversity and mapping studies in pearl millet (Bertin et al 2005), lupin (Phan et al 2007), etc.…”

Section: Intron Targeted Marker Development By Using Comparative Genomentioning

confidence: 99%

Gene-Based Marker Systems in Plants: High Throughput Approaches for Marker Discovery and Genotyping

Varshney

2009

Molecular Techniques in Crop Improvement

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Development and application of molecular markers derived from genes, commonly called genic markers or sometimes functional markers, is gaining momentum in plant genetics and breeding. Availability of large amount of sequence data coming from genome/transcriptome sequencing projects as well as advent of next generation sequencing technologies together with advances in bioinformatics tools, marker discovery is becoming cheaper and faster. The availability of inexpensive high-density SNP-genotyping arrays is encouraging the plant genetics and breeding community to undertake genome-wide marker genotyping for a variety of applications. For instance, high-throughput and low cost genotyping assays for gene-based markers offers the possibility to accelerate the trait mapping based on high-density linkage mapping as well as genome-scanning based association mapping approaches in addition to facilitate physical mapping, comparative mapping, phylogenetic studies and understanding genome organization in crop plant species. Marker discovery, genotyping and molecular breeding practices would be routine in near future for crop improvement in many crop species. Advances in the area of marker discovery and genotyping using highly parallel genomics assays and also a few applications have been discussed in this chapter.

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A Comparative Genomics Strategy for Targeted Discovery of Single-Nucleotide Polymorphisms and Conserved-Noncoding Sequences in Orphan Crops

Cited by 89 publications

References 35 publications

Construction of Genetic Linkage Map and QTL Analysis of Sink-Size Traits in Pearl Millet (Pennisetum glaucum)

Construction of Genetic Linkage Map and QTL Analysis of Sink-Size Traits in Pearl Millet (Pennisetum glaucum)

Striga

Gene-Based Marker Systems in Plants: High Throughput Approaches for Marker Discovery and Genotyping

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