Your search keyword '"Tadasu Shin-I"' showing total 3 results

1. Molecular cloning and characterization of the repetitive DNA sequences that comprise the constitutive heterochromatin of the W chromosomes of medaka fishes

Author

Asao Fujiyama, Yoichi Matsuda, Yuji Kohara, Tadasu Shin-I, Yusuke Asada, Satoshi Hamaguchi, Kiyoshi Naruse, Mitsuru Sakaizumi, and Yusuke Takehana

Subjects

Male, Heterochromatin, Oryzias, Molecular Sequence Data, Homology (biology), Species Specificity, RNA, Ribosomal, 28S, RNA, Ribosomal, 18S, Genetics, Animals, Constitutive heterochromatin, Cloning, Molecular, In Situ Hybridization, Fluorescence, Phylogeny, Repetitive Sequences, Nucleic Acid, Sex Chromosomes, Autosome, biology, Chromosome Mapping, Chromosome, Genes, rRNA, Sex Determination Processes, biology.organism_classification, W chromosome, Female, Oryzias javanicus

Abstract

Among the medaka fishes of the genus Oryzias, most species have homomorphic sex chromosomes, while some species, such as Oryzias hubbsi and Oryzias javanicus, have heteromorphic ZW sex chromosomes. In this study, a novel family of repetitive sequence was molecularly cloned from O. hubbsi and characterized by chromosome in situ and filter hybridization, respectively. This repetitive element, which we designated as a BstNI family element, localized at heterochromatin regions on the W chromosome, as well as on two pairs of autosomes. Homologous sequences to this element were found only in O. javanicus, which is a sister species of O. hubbsi, suggesting that this repeated element originated in the common ancestor of these two species. However, the intensity of the hybridization signals was lower in O. javanicus than in O. hubbsi, and the chromosomal location of this element in O. javanicus was confined to heterochromatin regions on one pair of autosomes. Thus, we hypothesize that this repetitive element was extensively amplified in the O. hubbsi lineage, especially on its W chromosome, after the separation of the O. javanicus lineage. In addition, we also found the W chromosomal location of the 18S-28S ribosomal RNA genes in both O. hubbsi and O. javanicus. Our previous studies showed no linkage homology of the sex chromosomes in these species, indicating that the RNA genes were shared between W chromosomes of different origins. This situation may be explained by a translocation of the sex-determining region with the ribosomal RNA genes in either species or an independent accumulation of the RNA genes as a convergent process during W chromosome degeneration.

Published

2011

2. Open-reading-frame sequence tags (OSTs) support the existence of at least 17,300 genes in C. elegans

Author

Michael A. Brasch, Lynn Doucette-Stamm, Jean Vandenhaute, Jean Thierry-Mieg, Nia Tzellas, Philippe Lamesch, Jérôme Reboul, Marc Vidal, Gary F. Temple, Tadasu Shin-I, Nicolas Thierry-Mieg, James L. Hartley, Troy Moore, Joseph Hitti, David E. Hill, Yuji Kohara, Cindy Jackson, Hongmei Lee, Danielle Thierry-Mieg, and Philippe Vaglio

Subjects

Expressed Sequence Tags, Genetics, Expressed sequence tag, Intron, Biology, biology.organism_classification, Polymerase Chain Reaction, Genome, Homology (biology), Open Reading Frames, Open reading frame, Species Specificity, Animals, Humans, ORFS, Caenorhabditis elegans, Gene, Genes, Helminth

Abstract

The genome sequences of Caenorhabditis elegans, Drosophila melanogaster and Arabidopsis thaliana have been predicted to contain 19,000, 13,600 and 25,500 genes, respectively. Before this information can be fully used for evolutionary and functional studies, several issues need to be addressed. First, the gene number estimates obtained in silico and not yet supported by any experimental data need to be verified. For example, it seems biologically paradoxical that C. elegans would have 50% more genes than Drosophilia. Second, intron/exon predictions need to be tested experimentally. Third, complete sets of open reading frames (ORFs), or "ORFeomes," need to be cloned into various expression vectors. To address these issues simultaneously, we have designed and applied to C. elegans the following strategy. Predicted ORFs are amplified by PCR from a highly representative cDNA library using ORF-specific primers, cloned by Gateway recombination cloning and then sequenced to generate ORF sequence tags (OSTs) as a way to verify identity and splicing. In a sample (n=1,222) of the nearly 10,000 genes predicted ab initio (that is, for which no expressed sequence tag (EST) is available so far), at least 70% were verified by OSTs. We also observed that 27% of these experimentally confirmed genes have a structure different from that predicted by GeneFinder. We now have experimental evidence that supports the existence of at least 17,300 genes in C. elegans. Hence we suggest that gene counts based primarily on ESTs may underestimate the number of genes in human and in other organisms.

Published

2001

3. Large-scale analysis of full-length cDNAs from the tomato (Solanum lycopersicum) cultivar Micro-Tom, a reference system for the Solanaceae genomics

Author

Naoki Yamamoto, Katsumi Yazawa, Nozomu Sakurai, Koh Aoki, Hiroshi Ezura, Kunihiro Suda, Sumire Fukushima, Daisuke Shibata, Ayako Suzuki, Yuichiro Watanabe, Akiko Okabe, Takanori Narita, Kentaro Yano, Tatsuya Suzuki, Motoichiro Kodama, Shingo Kawamura, Kazuhide Ooga, Mayumi Egusa, Manabu Watanabe, Taneaki Tsugane, Maiko Torii, Yuki Ichinose, Toshikazu Omura, Atsushi Kurabayashi, Tadasu Shin-I, Tsutomu Arie, Mari Kikuchi, Yuji Kohara, Yuko Sato, Shinobu Satoh, and Hideki Takahashi

Subjects

Molecular breeding, Genetics, Expressed sequence tag, DNA, Complementary, lcsh:QH426-470, DNA, Plant, biology, lcsh:Biotechnology, fungi, food and beverages, Genomics, biology.organism_classification, Genome, DNA sequencing, lcsh:Genetics, Solanum lycopersicum, lcsh:TP248.13-248.65, Solanum, Functional genomics, Gene, Research Article, Gene Library, Biotechnology

Abstract

Background The Solanaceae family includes several economically important vegetable crops. The tomato (Solanum lycopersicum) is regarded as a model plant of the Solanaceae family. Recently, a number of tomato resources have been developed in parallel with the ongoing tomato genome sequencing project. In particular, a miniature cultivar, Micro-Tom, is regarded as a model system in tomato genomics, and a number of genomics resources in the Micro-Tom-background, such as ESTs and mutagenized lines, have been established by an international alliance. Results To accelerate the progress in tomato genomics, we developed a collection of fully-sequenced 13,227 Micro-Tom full-length cDNAs. By checking redundant sequences, coding sequences, and chimeric sequences, a set of 11,502 non-redundant full-length cDNAs (nrFLcDNAs) was generated. Analysis of untranslated regions demonstrated that tomato has longer 5'- and 3'-untranslated regions than most other plants but rice. Classification of functions of proteins predicted from the coding sequences demonstrated that nrFLcDNAs covered a broad range of functions. A comparison of nrFLcDNAs with genes of sixteen plants facilitated the identification of tomato genes that are not found in other plants, most of which did not have known protein domains. Mapping of the nrFLcDNAs onto currently available tomato genome sequences facilitated prediction of exon-intron structure. Introns of tomato genes were longer than those of Arabidopsis and rice. According to a comparison of exon sequences between the nrFLcDNAs and the tomato genome sequences, the frequency of nucleotide mismatch in exons between Micro-Tom and the genome-sequencing cultivar (Heinz 1706) was estimated to be 0.061%. Conclusion The collection of Micro-Tom nrFLcDNAs generated in this study will serve as a valuable genomic tool for plant biologists to bridge the gap between basic and applied studies. The nrFLcDNA sequences will help annotation of the tomato whole-genome sequence and aid in tomato functional genomics and molecular breeding. Full-length cDNA sequences and their annotations are provided in the database KaFTom http://www.pgb.kazusa.or.jp/kaftom/ via the website of the National Bioresource Project Tomato http://tomato.nbrp.jp.

Published

2010