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High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice

Although quantitative traits loci (QTL) analysis has been widely performed to isolate agronomically important genes, it has been difficult to obtain molecular markers between individuals with similar phenotypes (assortative mating). Recently, the miniature inverted-repeat transposable element mPing...

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Autores principales: Monden, Yuki, Naito, Ken, Okumoto, Yutaka, Saito, Hiroki, Oki, Nobuhiko, Tsukiyama, Takuji, Ideta, Osamu, Nakazaki, Tetsuya, Wessler, Susan R., Tanisaka, Takatoshi
Formato: Texto
Lenguaje:English
Publicado: Oxford University Press 2009
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2671205/
https://www.ncbi.nlm.nih.gov/pubmed/19270311
http://dx.doi.org/10.1093/dnares/dsp004
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author Monden, Yuki
Naito, Ken
Okumoto, Yutaka
Saito, Hiroki
Oki, Nobuhiko
Tsukiyama, Takuji
Ideta, Osamu
Nakazaki, Tetsuya
Wessler, Susan R.
Tanisaka, Takatoshi
author_facet Monden, Yuki
Naito, Ken
Okumoto, Yutaka
Saito, Hiroki
Oki, Nobuhiko
Tsukiyama, Takuji
Ideta, Osamu
Nakazaki, Tetsuya
Wessler, Susan R.
Tanisaka, Takatoshi
author_sort Monden, Yuki
collection PubMed
description Although quantitative traits loci (QTL) analysis has been widely performed to isolate agronomically important genes, it has been difficult to obtain molecular markers between individuals with similar phenotypes (assortative mating). Recently, the miniature inverted-repeat transposable element mPing was shown to be active in the japonica strain Gimbozu EG4 where it had accumulated more than 1000 copies. In contrast, most other japonicas, including Nipponbare, have 50 or fewer mPing insertions in their genome. In this study we have exploited the polymorphism of mPing insertion sites to generate 150 PCR markers in a cross between the closely related japonicas, Nipponbare × Gimbozu (EG4). These new markers were distributed in genic regions of the whole genome and showed significantly higher polymorphism (150 of 183) than all other molecular markers tested including short sequence repeat markers (46 of 661). In addition, we performed QTL analysis with these markers using recombinant inbred lines derived from Nipponbare × Gimbozu EG4, and successfully mapped a locus involved in heading date on the short arm of chromosome 6. Moreover, we could easily map two novel loci involved in the culm length on the short arms of chromosomes 3 and 10.
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spelling pubmed-26712052009-05-22 High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice Monden, Yuki Naito, Ken Okumoto, Yutaka Saito, Hiroki Oki, Nobuhiko Tsukiyama, Takuji Ideta, Osamu Nakazaki, Tetsuya Wessler, Susan R. Tanisaka, Takatoshi DNA Res Full Papers Although quantitative traits loci (QTL) analysis has been widely performed to isolate agronomically important genes, it has been difficult to obtain molecular markers between individuals with similar phenotypes (assortative mating). Recently, the miniature inverted-repeat transposable element mPing was shown to be active in the japonica strain Gimbozu EG4 where it had accumulated more than 1000 copies. In contrast, most other japonicas, including Nipponbare, have 50 or fewer mPing insertions in their genome. In this study we have exploited the polymorphism of mPing insertion sites to generate 150 PCR markers in a cross between the closely related japonicas, Nipponbare × Gimbozu (EG4). These new markers were distributed in genic regions of the whole genome and showed significantly higher polymorphism (150 of 183) than all other molecular markers tested including short sequence repeat markers (46 of 661). In addition, we performed QTL analysis with these markers using recombinant inbred lines derived from Nipponbare × Gimbozu EG4, and successfully mapped a locus involved in heading date on the short arm of chromosome 6. Moreover, we could easily map two novel loci involved in the culm length on the short arms of chromosomes 3 and 10. Oxford University Press 2009-04 2009-03-06 /pmc/articles/PMC2671205/ /pubmed/19270311 http://dx.doi.org/10.1093/dnares/dsp004 Text en © The Author 2009. Kazusa DNA Research Institute.
spellingShingle Full Papers
Monden, Yuki
Naito, Ken
Okumoto, Yutaka
Saito, Hiroki
Oki, Nobuhiko
Tsukiyama, Takuji
Ideta, Osamu
Nakazaki, Tetsuya
Wessler, Susan R.
Tanisaka, Takatoshi
High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice
title High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice
title_full High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice
title_fullStr High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice
title_full_unstemmed High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice
title_short High Potential of a Transposon mPing as a Marker System in japonica × japonica Cross in Rice
title_sort high potential of a transposon mping as a marker system in japonica × japonica cross in rice
topic Full Papers
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2671205/
https://www.ncbi.nlm.nih.gov/pubmed/19270311
http://dx.doi.org/10.1093/dnares/dsp004
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