• 미생물학회지
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• 제29권5호
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• pp.284-289
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• 1991

the nucleotide sequence of the 3' terminal 568 bases of the 18S rRNA gene from Mucor racemosus was determined. The 3' end of the structural gene was identified by comparison with the published sequence for the Saccharomyces cerevisiae gene. The M. racemosus gene was found to share 83.8% homology with that of S. cerevisiae and 71-81% homology with those of human, mouse, maize, Xenopus laevis and Tetrahymena thermophila. The known methylation sites in X. laevis and human were also highly conserved in M. racemosus and located within most conserved regions of 18S RNA gene throughout evolution.

• 한국약용작물학회지
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• 제17권1호
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• pp.26-32
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• 2009

The region containing 18S rRNA gene, ITS 1 and part of the 5.8S rRNA gene of the Atractylodes japonica Koidz was amplified by PCR and the product cloned in a pBluescript SK II plasmid. DNA sequence of the cloned DNA was determined and submitted to the GenBank (accession number EU678363). Phylogenetic analysis of the ITS 1 DNA showed close similarity with the other plant species of the family Compositae. The extract of the plant materials of five different members of the family Compositae was analyzed by HPLC to detect atractylon. Extract of the A. japonica Koidz showed presence of significant amount of atractylon. However, noticeable amount of atractylon was not detected by the same analyses from the extracts of the other plants belonging to the family Compositae including Artemisia capillaris, Chrysantemum zawadskii, Eclipta prostrata or Taraxacum platycarpum.

• The Plant Pathology Journal
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• 제18권2호
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• pp.98-101
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• 2002

Using phytoplasma universal primer pair Pl and P7, a fragment of about 1.8 kb nucleotide sequences of 16S rRNA gene and 16S-23S rRNA intergenic spacer region, and a portion of 23S rRNA gene of jujube witches'broom (JWB) and mulberry dwarf(MD) phytoplasmas were determined. The nucleotide sequences of JWB and MD were 1,850 bp and 1,831 bp long, respectively. The JWB phytoplasma sequence was aligned with the homologous sequence of MD phytoplasma. Twenty-eight base insertions and nine base deletions were found in the JWB phytoplasma sequence compared with that of MD phytoplasma. The similarity of the aligned sequences of JWB and MD was 84.8%. The near-complete 16S rRNA gene DNA sequences of JWB and MD were 1,529 bp and 1,530 bp in length, respectively, and revealed 89.0% homology. The 16S-23S rRNA intergenic spacer region DNA sequences were 263 bp and 243 bp in lengths respectively, while homology was only 70% and the conserved tRNA-lle gene of JWB and MD was located into the intergenic space region between 16S-23S rRNA gene. The nucleotide sequences were 77 bp long in both JWB and MD, and showed 97.4% sequence homology. Based on the phylogenetic analysis of the two phytoplasmas, the JWB phytoplasma belongs to the Elm yellow phytoplasma group (16S rV), whereas, the MD phytoplasma belongs to the Aster yellow group (16S rI).

• Parasites, Hosts and Diseases
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• 제51권4호
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• pp.401-412
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• 2013

Because of an increased number of Acanthamoeba keratitis (AK) along with associated disease burdens, medical professionals have become more aware of this pathogen in recent years. In this study, by analyzing both the nuclear 18S small subunit ribosomal RNA (18S rRNA) and mitochondrial 16S rRNA gene loci, 27 clinical Acanthamoeba strains that caused AK in Japan were classified into 3 genotypes, T3 (3 strains), T4 (23 strains), and T5 (one strain). Most haplotypes were identical to the reference haplotypes reported from all over the world, and thus no specificity of the haplotype distribution in Japan was found. The T4 sub-genotype analysis using the 16S rRNA gene locus also revealed a clear subconformation within the T4 cluster, and lead to the recognition of a new sub-genotype T4i, in addition to the previously reported sub-genotypes T4a-T4h. Furthermore, 9 out of 23 strains in the T4 genotype were identified to a specific haplotype (AF479533), which seems to be a causal haplotype of AK. While heterozygous nuclear haplotypes were observed from 2 strains, the mitochondrial haplotypes were homozygous as T4 genotype in the both strains, and suggested a possibility of nuclear hybridization (mating reproduction) between different strains in Acanthamoeba. The nuclear 18S rRNA gene and mitochondrial 16S rRNA gene loci of Acanthamoeba spp. possess different unique characteristics usable for the genotyping analyses, and those specific features could contribute to the establishment of molecular taxonomy for the species complex of Acanthamoeba.

• Animal Systematics, Evolution and Diversity
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• nspc3호
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• pp.139-146
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• 1992

중합효소연쇄반응(PCR)을 이용한 클로닝 기법과 Taq 염기서열분석법을 사용하여 갑각류에 속하는 뿔물맞이게(Pugettia quadridens)(십각 목, 범배 아목, 게 하목)에 대한 18S 리보솜 RNA 유전자의 1차염기서열을 밝혔다. 본 종의 18S 리보솜 RNA 유전자는 십각류에 속하는 또 다른 종인 두드러기어리게(Oedignathus inermis)보다 46개가 짧은 1837개의 염기로 이루어져 있었다. 염기가 삽입되거나 결실된 부분을 고려하지 않았을때에 두 종간에 염기서열 유사도는 90.8%이었다. 염기서열이 가장 보존적인 부위는 1137-1206(70개) 분위로 이 부위에서는 두 종이 완전히 동일한 염기서열을 보이고 있었고, 변이가 연속적으로 가장 큰 부위는 46-55 부위였고 399-407 부위가 그 다음으로 많은 연속적 변이를 가지고 있었다. 18S 리보솜 RNA 유전자의 1차구조에 있어서 염기서열의 변이는 이 유전자 전체를 통해 고르게 분포하지 않았다.

• Parasites, Hosts and Diseases
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• 제60권4호
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• pp.295-299
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• 2022

Malaria elimination and control require prompt and accurate diagnosis for treatment plan. Since microscopy and rapid diagnostic test (RDT) are not sensitive particularly for diagnosing low parasitemia, highly sensitive diagnostic tools are required for accurate treatment. Molecular diagnosis of malaria is commonly carried out by nested polymerase chain reaction (PCR) targeting 18S rRNA gene, while this technique involves long turnaround time and multiple steps leading to false positive results. To overcome these drawbacks, we compared highly sensitive cytochrome oxidase gene-based single-step multiplex reaction with 18S rRNA nested PCR. Cytochrome oxidase (cox) genes of P. falciparum (cox-III) and P. vivax (cox-I) were compared with 18S rRNA gene nested PCR and microscopy. Cox gene multiplex PCR was found to be highly specific and sensitive, enhancing the detection limit of mixed infections. Cox gene multiplex PCR showed a sensitivity of 100% and a specificity of 97%. This approach can be used as an alternative diagnostic method as it offers higher diagnostic performance and is amenable to high throughput scaling up for a larger sample size at low cost.

• 대한본초학회지
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• 제21권2호
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• pp.9-13
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• 2006

Objectives : To determine the DNA sequence of the 18S rRNA gene of the Rehmannia glutinosa and analyze it phylogenetically Methods : Dried root of the Rehmannia glutinosa was ground with a mortar and pestle. Glass beads(0.5 mm in diameter), TE buffer and SDS solution were added to that. The mixture was vortexed vigorously and extracted with the mixture of phenol, chloroform and isoamyl alcohol and with the mixture of the chloroform and isoamyl alcohol. The nucleic acids were precipitated with ethanol and resuspended in TE buffer. Contaminating RNA was digested with RNAse A and the DNA was purified further with the Geneclean Turbo Kit. This DNA was used as a template for amplification of the 18S rRNA gene by PCR. The PCR product was cloned in the pBluescript SK II plasmid by blunt-end ligation and the DNA sequence of the insert was determined. This DNA sequence was analyzed phylogenetically by the BLAST program. Results and Conclusion : Vortexing the ground powder of the dried plant root with glass beads during cell lysis improved recovery of DNA. The DNA sequence of the Rehmannia glutinosa 18S rRNA gene was determined and deposited at the GenBank as the accession number DQ469606. Phylogenetic analysis of that sequence showed the relationship between the members of the family of Scrophulariaceae and also the close relationship of the Buddleja davidii to the members of the Scrophulariaceae family.

• 한국동물학회지
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• 제37권3호
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• pp.343-351
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• 1994

The partial nucleotide sequences of 185 ribosomal RNA gene were compared for six cnidarian species (one belongs to class Hvdrozoa: Coryne pusilla. Five belong to class Anthozoa: Beflonella rigida from Octocorallia; Anemonia sulcutu, Anthopfeura kurognne, An thopleura midori from Hexacorallia: Cerianthus filiformis from Ceriantipatharial. The aligned sequence data were used to test the hypothesis on the anthozoan phylosenv by using the distance matrix method and parsimony method. The phvlosenetic inferences resulting from these methods indicate that the anthozoan is a monophvletic group and support the three subclass scheme (Octocorallia, HexBcorallia, Ceriantipatharial within class Anthozoa. The result also indicates that ceriantipatharian is more primitive than the other groups and that family Actiniidae is a monophvletic group within the anthozoan. However, the present analysis does not clearly indicate the phvlogenetic relationships of species among genera.

• 생명과학회지
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• 제22권2호
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• pp.167-176
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• 2012

발효가 진행중인 멸치액젓에서 단백질분해효소를 생산하는 3종의 호염성 세균을 분리하였다. 분리된 FAM 10, FAM 114, 그리고 FAM 115는 각각 소금농도가 2~4%, 10%, 6%에서 최적 세포성장이 관찰되었으며, 18~22% 소 금농도까지 생육이 가능했다. 단백질분해효소 생산을 위한 최적 소금농도는 FAM 10은 6%, FAM 114와 FAM 115는 10%로 나타났다. FAM 10의 단백질분해효소 활성은 10%까지 첨가하면 서서히 저하되며, 14% 소금농도에서는 효소활성이 없는 반면, FAM 114와 FAM 115의 경우, 14%까지 효소활성을 나타냈으며 18%에서는 활성을 관찰할 수 없었다. 이러한 결과로부터 분리된 3종의 미생물이 중간 정도의 호염성 세균임을 증명하였다. 16S rRNA 유전자와 16S-23S 유전자 사이 공간(IGS) 서열, 생화학적 실험, 그람염색을 이용하여 비교 분석한 결과, FAM 10, FAM 114, 그리고 FAM 115는 각각 Salinivibrio sp., Halobacillus sp., 그리고 Halobacillus sp.임을 동정하였다. Salinivibrio sp. FAM 10에는 191번째 서열부터 약간 다른 2가지 종류의 16S rDNA와 16S-23S IGS내에 tRNA 유전자가 없는 형태, 이소루이신/알라닌, 글루탐산/라이신/발린을 운반하는 tRNA 유전자들을 함유하는 4가지 종류의 다른 16S-23S IGS가 존재하였다. Hablobacillus sp. FAM 114와 FAM 115는 완전히 동일한 16S rRNA 유전자 서열을 가지고 있었으며, 여러 Halobacillus sp.와 99% 서열동일성을 보여주었다. IGS의 경우, tRNA 유전자가 없는 IGS와 이소루이신/알라닌을 운반하는 tRNA 유전자들을 함유하는 3가지 16S-23S IGS가 존재하였으며, Halobacillus aidingensis와 Halobacillus sp. JM-Hb의 IGS와 99% 서열동일성을 보여주었다.

• 한국수산과학회지
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• 제48권5호
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• pp.731-738
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• 2015

Nematode infection in the epithelial tissue of cultured rockfish Sebastes schlegeli was first reported in 2012. Since then, nematode infections have caused serious economic losses in rockfish aquaculture on the west coast of Korea. Taxonomic and life cycle information for this parasite are currently unknown. In this study, 18S rRNA and cytochrome c oxidase subunit I (COI) genes were used for molecular identification and polymerase chain reaction (PCR) to detect the invisible stages of this parasite. Nucleotide sequences of the 18S rRNA of the rockfish nematode showed 98% identity with that of Philometra morii. Therefore, this rockfish nematode was classified to the Philometridae family. However, we could not identify it to genus level using 18S rRNA. Its COI nucleotide sequences shared 85% and 82% identities with those of Bursaphelenchus sinensis and Philometra overstreeti, respectively. In addition, two gene-specific primer sets were designed based on the 18S rRNA gene to detect the intermediate host and nematode larvae. These primers were specific to this rockfish nematode without cross-reacting to other pathogens. The detection limit of the PCR assay using these primers was 1,000 copies of nematoda plasmid DNA. Therefore, the PCR assay described here is suitable for the detection of nematode DNA within rockfish. In addition, this PCR assay could be used to detect nematode larvae and the intermediate host.