Search

Your search keyword '"Tragoonrung S"' showing total 11 results
Start Over Author "Tragoonrung S" Search Limiters Peer Reviewed
11 results on '"Tragoonrung S"'

4. Microsatellite markers flanking the tms2 gene facilitated tropical TGMS rice line development

Author

Lopez, M.T., Toojinda, T., Vanavichit, A., and Tragoonrung, S.

Subjects
Rice -- Research, Agricultural industry, Business
Abstract

The use of thermosensitive genetic male sterility (TGMS) in the development and production of rice (Oryza sotiva L.) hybrids is an alternative to the cytoplasmic-genetic male sterility (CMS) system. This study aimed to develop TGMS lines with aromatic Thai rice background by molecular marker-aided breeding. Four microsatellite markers (RM2, RM10, RM11, and RM214) on chromosome 7 in the vicinity of the TGMS gene tms2 and showing polymorphism between the two parents were used in genotyping the mapping population consisting of 157 [F.sub.2] plants derived from a cross between Norin PL12 (a TGMS line from Japan) and KDML 105 (a popular aromatic Thai rice cultivar). The RMU marker was approximately 5 centimorgans (cM) from tms2 while RM2 was approximately 16 cM from it. In this [F.sub.2] population, the accuracy of selecting sterile plants with RM2 and RMI1 markers was 92 and 97%, respectively. In three backcrosses, the accuracy of selection with markers for either homozygous or heterozygous plants was higher than 90% with RM2. Using RM11, we obtained 89% accuracy for selecting homozygous fertile plants and 59% accuracy for selecting heterozygous plants. The results demonstrated that microsatellite markers were powerful in screening large breeding populations, and these markers facilitated selection for plants possessing the tms2 in an early stage of the crop and without exposing the materials to the required temperature for TGMS gene expression. Three TGMS lines with aromatic Thai rice background were developed and showed complete pollen sterility when maximum temperature was higher than 30°C, 1 to 2 wk after panicle initiation. Up to 77% spikelet fertility was observed when these lines were exposed at temperature below 30°C during the critical stage., HYBRID RICE TECHNOLOGY has tremendously improved rice productivity as effectively demonstrated in China and other Asian countries. To date, the CMS or three-line method is effective and widely used in [...]

Published
2003

6. The Chloroplast Genome Sequence of Mungbean (Vigna radiata) Determined by High-throughput Pyrosequencing: Structural Organization and Phylogenetic Relationships.

Author

Tangphatsornruang, S., Sangsrakru, D., Chanprasert, J., Uthaipaisanwong, P., Yoocha, T., Jomchai, N., and Tragoonrung, S.

Abstract

Mungbean is an economically important crop which is grown principally for its protein-rich dry seeds. However, genomic research of mungbean has lagged behind other species in the Fabaceae family. Here, we reported the complete chloroplast (cp) genome sequence of mungbean obtained by the 454 pyrosequencing technology. The mungbean cp genome is 151 271 bp in length which includes a pair of inverted repeats (IRs) of 26 474 bp separated by a small single-copy region of 17 427 bp and a large single-copy region of 80 896 bp. The genome contains 108 unique genes and 19 of these genes are duplicated in the IR. Of these, 75 are predicted protein-coding genes, 4 ribosomal RNA genes and 29 tRNA genes. Relative to other plant cp genomes, we observed two distinct rearrangements: a 50-kb inversion between accD/rps16 and rbcL/trnK-UUU, and a 78-kb rearrangement between trnH/rpl14 and rps19/rps8. We detected sequence length polymorphism in the cp homopolymeric regions at the intra- and inter-specific levels in the Vigna species. Phylogenetic analysis demonstrated a close relationship between Vigna and Phaseolus in the phaseolinae subtribe and provided a strong support for a monophyletic group of the eurosid I. [ABSTRACT FROM PUBLISHER]

Published
2010
Full Text
View/download PDF

7. Feasibility of using 454 pyrosequencing for studying quasispecies of the whole dengue viral genome

Author

Chin-inmanu Kwanrutai, Suttitheptumrong Aroonroong, Sangsrakru Duangjai, Tangphatsornruang Sithichoke, Tragoonrung Somvong, Malasit Prida, Tungpradabkul Sumalee, and Suriyaphol Prapat

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background Dengue is the world's most common mosquito-borne viral disease. Poor proofreading by RNA polymerase during its replication results in the accumulation of mutations in its genome. This leads to a diversity of genotypes in the viral population termed quasispecies. Quasispecies play an important role in disease severity. The study of quasispecies in dengue has been hindered because of the requirement for large amounts of cloning and sequencing, which could be overcome by 454 pyrosequencing. In this study, we attempted to demonstrate the feasibility of using 454 pyrosequencing to study genome diversity of dengue virus quasispecies by sequencing a pool of known dengue viral strains. Results Two sets of dengue DNA templates were sequenced by 454/Roche GS FLX. The total number of reads for data 1 and data 2 were 54,440 and 134,441, with average lengths of 221 and 232 bp, respectively. Reads containing ambiguous base Ns were excluded (6.00% in data 1, 7.05% in data 2). More than 99% of reads could be aligned back to the correct serotypes by BLAST. The reads covered the whole genome without any gaps, and the minimum coverage depth was 50×. Frequencies of known strains detected from each data set were highly correlated with the input ratios. We also explored criteria for filtering error reads and artifacts from true variations. Conclusions This study showed that 454 pyrosequencing, coupled with our analysis procedure, could sequence the whole genome of dengue virus with good coverage. The ratio of detected variants in the sequencing data reflected the starting ratio, proving that the proposed technique could be used to study the frequencies of variants in quasispecies.

Published
2012
Full Text
View/download PDF

8. Temporal and spatial expression of polygalacturonase gene family members reveals divergent regulation during fleshy fruit ripening and abscission in the monocot species oil palm

Author

Roongsattham Peerapat, Morcillo Fabienne, Jantasuriyarat Chatchawan, Pizot Maxime, Moussu Steven, Jayaweera Dasuni, Collin Myriam, Gonzalez-Carranza Zinnia H, Amblard Philippe, Tregear James W, Tragoonrung Somvong, Verdeil Jean-Luc, and Tranbarger Timothy J

Subjects
Abscission, Fruit development, Elaeis guineensis, Polygalacturonase, Ethylene, Cell separation, Botany, QK1-989
Abstract

Abstract Background Cell separation that occurs during fleshy fruit abscission and dry fruit dehiscence facilitates seed dispersal, the final stage of plant reproductive development. While our understanding of the evolutionary context of cell separation is limited mainly to the eudicot model systems tomato and Arabidopsis, less is known about the mechanisms underlying fruit abscission in crop species, monocots in particular. The polygalacturonase (PG) multigene family encodes enzymes involved in the depolymerisation of pectin homogalacturonan within the primary cell wall and middle lamella. PG activity is commonly found in the separation layers during organ abscission and dehiscence, however, little is known about how this gene family has diverged since the separation of monocot and eudicots and the consequence of this divergence on the abscission process. Results The objective of the current study was to identify PGs responsible for the high activity previously observed in the abscission zone (AZ) during fruit shedding of the tropical monocot oil palm, and to analyze PG gene expression during oil palm fruit ripening and abscission. We identified 14 transcripts that encode PGs, all of which are expressed in the base of the oil palm fruit. The accumulation of five PG transcripts increase, four decrease and five do not change during ethylene treatments that induce cell separation. One PG transcript (EgPG4) is the most highly induced in the fruit base, with a 700–5000 fold increase during the ethylene treatment. In situ hybridization experiments indicate that the EgPG4 transcript increases preferentially in the AZ cell layers in the base of the fruit in response to ethylene prior to cell separation. Conclusions The expression pattern of EgPG4 is consistent with the temporal and spatial requirements for cell separation to occur during oil palm fruit shedding. The sequence diversity of PGs and the complexity of their expression in the oil palm fruit tissues contrast with data from tomato, suggesting functional divergence underlying the ripening and abscission processes has occurred between these two fruit species. Furthermore, phylogenetic analysis of EgPG4 with PGs from other species suggests some conservation, but also diversification has occurred between monocots and eudicots, in particular between dry and fleshy fruit species.

Published
2012
Full Text
View/download PDF

9. SSR markers in transcripts of genes linked to post-transcriptional and transcriptional regulatory functions during vegetative and reproductive development of Elaeis guineensis

Author

Tranbarger Timothy, Kluabmongkol Wanwisa, Sangsrakru Duangjai, Morcillo Fabienne, Tregear James W, Tragoonrung Somvong, and Billotte Norbert

Subjects
Botany, QK1-989
Abstract

Abstract Background The oil palm (Elaeis guineensis Jacq.) is a perennial monocotyledonous tropical crop species that is now the world's number one source of edible vegetable oil, and the richest dietary source of provitamin A. While new elite genotypes from traditional breeding programs provide steady yield increases, the long selection cycle (10-12 years) and the large areas required to cultivate oil palm make genetic improvement slow and labor intensive. Molecular breeding programs have the potential to make significant impacts on the rate of genetic improvement but the limited molecular resources, in particular the lack of molecular markers for agronomic traits of interest, restrict the application of molecular breeding schemes for oil palm. Results In the current study, 6,103 non-redundant ESTs derived from cDNA libraries of developing vegetative and reproductive tissues were annotated and searched for simple sequence repeats (SSRs). Primer pairs from sequences flanking 289 EST-SSRs were tested to detect polymorphisms in elite breeding parents and their crosses. 230 of these amplified PCR products, 88 of which were polymorphic within the breeding material tested. A detailed analysis and annotation of the EST-SSRs revealed the locations of the polymorphisms within the transcripts, and that the main functional category was related to transcription and post-transcriptional regulation. Indeed, SSR polymorphisms were found in sequences encoding AP2-like, bZIP, zinc finger, MADS-box, and NAC-like transcription factors in addition to other transcriptional regulatory proteins and several RNA interacting proteins. Conclusions The identification of new EST-SSRs that detect polymorphisms in elite breeding material provides tools for molecular breeding strategies. The identification of SSRs within transcripts, in particular those that encode proteins involved in transcriptional and post-transcriptional regulation, will allow insight into the functional roles of these proteins by studying the phenotypic traits that cosegregate with these markers. Finally, the oil palm EST-SSRs derived from vegetative and reproductive development will be useful for studies on the evolution of the functional diversity within the palm family.

Published
2012
Full Text
View/download PDF

10. Characterization of microsatellites and gene contents from genome shotgun sequences of mungbean (Vigna radiata (L.) Wilczek)

Author

Sommanas Warunee, Seehalak Worapa, Sangsrakru Duangjai, Chanprasert Juntima, Uthaipaisanwong Pichahpuk, Somta Prakit, Tangphatsornruang Sithichoke, Tragoonrung Somvong, and Srinives Peerasak

Subjects
Botany, QK1-989
Abstract

Abstract Background Mungbean is an important economical crop in Asia. However, genomic research has lagged behind other crop species due to the lack of polymorphic DNA markers found in this crop. The objective of this work is to develop and characterize microsatellite or simple sequence repeat (SSR) markers from genome shotgun sequencing of mungbean. Result We have generated and characterized a total of 470,024 genome shotgun sequences covering 100.5 Mb of the mungbean (Vigna radiata (L.) Wilczek) genome using 454 sequencing technology. We identified 1,493 SSR motifs that could be used as potential molecular markers. Among 192 tested primer pairs in 17 mungbean accessions, 60 loci revealed polymorphism with polymorphic information content (PIC) values ranging from 0.0555 to 0.6907 with an average of 0.2594. Majority of microsatellite markers were transferable in Vigna species, whereas transferability rates were only 22.90% and 24.43% in Phaseolus vulgaris and Glycine max, respectively. We also used 16 SSR loci to evaluate phylogenetic relationship of 35 genotypes of the Asian Vigna group. The genome survey sequences were further analyzed to search for gene content. The evidence suggested 1,542 gene fragments have been sequence tagged, that fell within intersected existing gene models and shared sequence homology with other proteins in the database. Furthermore, potential microRNAs that could regulate developmental stages and environmental responses were discovered from this dataset. Conclusion In this report, we provided evidence of generating remarkable levels of diverse microsatellite markers and gene content from high throughput genome shotgun sequencing of the mungbean genomic DNA. The markers could be used in germplasm analysis, accessing genetic diversity and linkage mapping of mungbean.

Published
2009
Full Text
View/download PDF

11. Characterization of the chloroplast genome sequence of oil palm (Elaeis guineensis Jacq.)

Author

Uthaipaisanwong, P., Chanprasert, J., Shearman, J.R., Sangsrakru, D., Yoocha, T., Jomchai, N., Jantasuriyarat, C., Tragoonrung, S., and Tangphatsornruang, S.

Subjects
*CHLOROPLAST DNA, *AMINO acid sequence, *OIL palm, *NUCLEOTIDE sequence, *RIBOSOMAL RNA, *MONOCOTYLEDONS, *PLANT genomes
Abstract

Abstract: Oil palm (Elaeis guineensis Jacq.) is an economically important crop, which is grown for oil production. To better understand the molecular basis of oil palm chloroplasts, we characterized the complete chloroplast (cp) genome sequence obtained from 454 pyrosequencing. The oil palm cp genome is 156,973bp in length consisting of a large single-copy region of
85,192bp flanked on each side by inverted repeats of 27,071bp with a small single-copy region of 17,639bp joining the
repeats. The genome contains 112 unique genes: 79 protein-coding genes, 4 ribosomal RNA genes and 29 tRNA genes. By aligning the cp
genome sequence with oil palm cDNA sequences, we observed 18 non-silent and 10 silent RNA editing events among 19 cp protein-coding genes. Creation of an initiation codon by RNA editing in rpl2 has been reported in several monocots and was also found in the oil palm cp genome. Fifty common chloroplast protein-coding genes from 33 plant taxa were used to construct ML and MP
phylogenetic trees. Their topologies are similar and strongly support for the position of E. guineensis as the sister of closely related species Phoenix dactylifera in Arecaceae (palm families) of monocot subtrees. [Copyright &y& Elsevier]

Published
2012
Full Text
View/download PDF

Catalog

Books, media, physical & digital resources
See catalog results