BackgroundA dinoflagellate genus Ostreopsis is known as a potential producer of Palytoxin derivatives. Palytoxin is the most potent non-proteinaceous compound reported so far. There has been a growing number of reports on palytoxin-like poisonings in southern areas of Japan; however, the distribution of Ostreopsis has not been investigated so far. Morphological plasticity of Ostreopsis makes reliable microscopic identification difficult so the employment of molecular tools was desirable.Methods/Principal FindingIn total 223 clones were examined from samples mainly collected from southern areas of Japan. The D8–D10 region of the nuclear large subunit rDNA (D8–D10) was selected as a genetic marker and phylogenetic analyses were conducted. Although most of the clones were unable to be identified, there potentially 8 putative species established during this study. Among them, Ostreopsis sp. 1–5 did not belong to any known clade, and each of them formed its own clade. The dominant species was Ostreopsis sp. 1, which accounted for more than half of the clones and which was highly toxic and only distributed along the Japanese coast. Comparisons between the D8–D10 and the Internal Transcribed Spacer (ITS) region of the nuclear rDNA, which has widely been used for phylogenetic/phylogeographic studies in Ostreopsis, revealed that the D8–D10 was less variable than the ITS, making consistent and reliable phylogenetic reconstruction possible.Conclusions/SignificanceThis study unveiled a surprisingly diverse and widespread distribution of Japanese Ostreopsis. Further study will be required to better understand the phylogeography of the genus. Our results posed the urgent need for the development of the early detection/warning systems for Ostreopsis, particularly for the widely distributed and strongly toxic Ostreopsis sp. 1. The D8–D10 marker will be suitable for these purposes.
Monitoring of harmful algal bloom (HAB) species in coastal waters is important for assessment of environmental impacts associated with HABs. Co-occurrence of multiple cryptic species such as toxic dinoflagellate Ostreopsis species make reliable microscopic identification difficult, so the employment of molecular tools is often necessary. Here we developed new qPCR method by which cells of cryptic species can be enumerated based on actual gene number of target species. The qPCR assay targets the LSU rDNA of Ostreopsis spp. from Japan. First, we constructed standard curves with a linearized plasmid containing the target rDNA. We then determined the number of rDNA copies per cell of target species from a single cell isolated from environmental samples using the qPCR assay. Differences in the DNA recovery efficiency was calculated by adding exogenous plasmid to a portion of the sample lysate before and after DNA extraction followed by qPCR. Then, the number of cells of each species was calculated by division of the total number of rDNA copies of each species in the samples by the number of rDNA copies per cell. To test our procedure, we determined the total number of rDNA copies using environmental samples containing no target cells but spiked with cultured cells of several species of Ostreopsis. The numbers estimated by the qPCR method closely approximated total numbers of cells added. Finally, the numbers of cells of target species in environmental samples containing cryptic species were enumerated by the qPCR method and the total numbers also closely approximated the microscopy cell counts. We developed a qPCR method that provides accurate enumeration of each cryptic species in environments. This method is expected to be a powerful tool for monitoring the various HAB species that occur as cryptic species in coastal waters.
Many genes are temporally and spatially regulated during embryogenesis in higher plants. Although many studies have examined transcriptional factors relating to gene regulation during embryogenesis, the molecular mechanisms relating to the initiation of embryogenesis are still unclear. In animals, it was reported that gene regulation by chromatin remodeling contributes to embryogenesis. In contrast, the relationship between chromatin remodeling and the initiation of embryogenesis in higher plants remains to be determined. LEAFY COTYLEDON1 (LEC1) is an important factor in early embryogenesis and is ectopically expressed in the pkl1-1 mutant, which is deficient in chromatin remodeling factor. Therefore, there is a high probability that chromatin remodeling regulates the expression of LEC1. To confirm this possibility, the histone methylation level, which is involved in chromatin remodeling, was examined for the genomic region of LEC1 by chromatin immunoprecipitation analysis. In the promoter region of LEC1, methylation of histone H3 lysine 4 in somatic embryos was higher in rosette leaves. SET domain-containing proteins are an important factor in histone methylation. To isolate the SET domain-containing protein genes (SET gene) involved in Arabidopsis thaliana embryogenesis, expression analyses using RT-PCR were performed. Among 37 SET genes, seven were found to have a high probability of involvement in embryogenesis.
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