• Parasites, Hosts and Diseases
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• 제51권3호
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• pp.353-355
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• 2013

There are approximately 20 known species of the genus Cryptosporidium, and among these, 8 infect immunocompetent or immunocompromised humans. C. hominis and C. parvum most commonly infect humans. Differentiating between them is important for evaluating potential sources of infection. We report here the development of a simple and accurate real-time PCR-based restriction fragment length polymorphism (RFLP) method to distinguish between C. parvum and C. hominis. Using the CP2 gene as the target, we found that both Cryptosporidium species yielded 224 bp products. In the subsequent RFLP method using TaqI, 2 bands (99 and 125 bp) specific to C. hominis were detected. Using this method, we detected C. hominis infection in 1 of 21 patients with diarrhea, suggesting that this method could facilitate the detection of C. hominis infections.

• The Plant Pathology Journal
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• 제26권4호
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• pp.321-327
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• 2010

We performed diagnostic PCR assays and a phylogenetic analysis using partial sequences of TEF1 (translation elongation factor-1) to determine the trichothecene chemotypes and genetic diversity of F. graminearum isolates from maize and rice samples collected in 2009 in Korea. PCR using a species-specific primer set revealed a total of 324 isolates belonging to the putative F. graminearum species complex. PCR with trichothecene chemotypespecific primers revealed that the nivalenol (NIV) chemotype was predominant among the fungal isolates from rice (95%) in all provinces examined. In contrast, the predominant chemotype among the corn isolates varied according to region. The deoxynivalenol (DON) chemotype was found more frequently (66%) than the NIV chemotype in Gangwon Province, whereas the NIV chemotype (70%) was predominant in Chungbuk Province. Phylogenetic analysis showed that all DON isolates examined were clustered into lineage 7, while the NIV isolates resided within lineage 6 (F. asiaticum). Compared with previous studies, the lineage 6 isolates in rice have been predominantly maintained in southern provinces, while the dominance of lineage 7 in maize has been evident in Gangwon at a slightly reduced level.

• 한국발생생물학회지:발생과생식
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• 제23권3호
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• pp.297-304
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• 2019

The higher fragment sizes (>2,100 bp) are not observed in the two C. spp. populations. The six oligonucleotides primers OPA-11, OPB-09, OPB-14, OPB-20, OPC-14, and OPC-18 were used to generate the unique shared loci to each tonguesole population and shared loci by the two tonguesole populations. The hierarchical polar dendrogram indicates two main clusters: Gunsan (GUNSAN 01-GUNSAN 11) and the Atlantic (ATLANTIC 12-ATLANTIC 22) from two geographic populations of tonguesoles. The shortest genetic distance displaying significant molecular difference was between individuals' GUNSAN no. 02-GUNSAN no. 01 (genetic distance=0.038). In the long run, individual no. 02 of the ATLANTIC tonguesole was most distantly related to GUNSAN no. 06 (genetic distance=0.958). These results demonstrate that the Gunsan tonguesole population is genetically different from the Atlantic tonguesole population. The potential of PCR analysis to identify diagnostic markers for the identification of two tonguesole populations has been demonstrated. As a rule, using various oligonucleotides primers, this PCR method has been applied to identify polymorphic/specific markers particular to species and geographical population, as well as genetic diversity/polymorphism in diverse species of organisms.

• Journal of Applied Biological Chemistry
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• 제52권1호
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• pp.1-7
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• 2009

후대교배종 CM 벼의 정성 PCR 검정방법을 개발하기 위하여, 벼의 내재유전자로써 OsCs-J(rice cytochrome c gene)을 선발하여 OsCytC-5'/3'의 primer쌍을 제작하고, 벼를 포함한 서로 다른 8개 작물에 대하여 PCR을 수행한 결과 벼에 특이적으로 증폭되는 111 bp의 반응 산물을 확인하였다. 국내 개발된 LS28$\times$CryIAc1 GM 벼의 검정 분석으로 정성 PCR 반응을 수행하였다. 정성 PCR을 위하여 GM 벼에 도입된 T-DNA 및 게놈상의 도입유전자 삽입부위의 인접서열을 바탕으로 구조 및 계통 특이적인 검정 primer 쌍을 제작하였다. ActCk-5'/3' primer 쌍을 이용하여 LS28의 T-DNA 내의 actin 프로모터와 OsCK1 유전자 사이를 증폭시켜 306 bp의 PCR 반응 산물을 얻을 수 있었으며, 또한 계통특이 primer 쌍인 CryIAc1 GM 벼유래의 CrLB-5'/3' 및 LS28 GM 벼 유래의 CKRB-5'/3'를 이용한 PCR 반응으로 각각 142 bp와 91 bp의 도입유전자의 인접서열 부위의 특이적인 증폭 산물을 확인할 수 있었다. 계통 특이적 검정을 위한 이들 개발 primer 쌍들은 event 계통과 대조적으로 non-GM 벼와 다양한 작물에 대하여 어떠한 특이적인 PCR 증폭 산물을 형성하지 않았다. 따라서 본 연구에서 계통특이 primer를 이용하여 후대교배종 GM 벼 계통, L528$\times$CryIAc1을 특이적으로 검출할 수 있음을 확인하였고, 제시된 방법이 GM 벼의 실용화를 위한 위해성평가의 검정방법 자료로 제공될 수 있음을 확인하였다.

• 생태와환경
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• 제54권3호
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• pp.209-220
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• 2021

Pacific herring, Clupea pallasii, a keystone species with significant ecological and commercial importance, is declining globally throughout much of its range. While traditional fishing equipment methods remain limited, new sensitive and rapid detection methods should be developed to monitor fisheries resources. To monitor the presence and quantity of C. pallasii from environmental DNA (eDNA) extracted from seawater samples, a pair of primers and a TaqMan^® probe specific to this fish based on mitochondrial cytochrome b (COB) sequences were designed for the real-time PCR (qPCR) assay. The combination of our molecular markers showed high specificity in the qPCR assay, which affirmed the success of presenting a positive signal only in the C. pallasii specimens. The markers also showed a high sensitivity for detecting C. pallasii genomic DNA in the range of 1 pg~100 ng rxn^-1 and its DNA plasmid containing COB amplicon in the range of 1~100,000copies rxn^-1, which produced linear standard calibration curves (r²=0.99). We performed a qPCR assay for environmental water samples obtained from 29 sampling stations in the southeastern coastal regions of South Korea using molecular markers. The assay successfully detected the C. pallasii eDNA from 14 stations (48.2%), with the highest mean concentration in Jinhae Bay with a value of 76.09±18.39 pg L^-1 (246.20±58.58 copies L^-1). Our preliminary application of molecular monitoring of C. pallasii will provide essential information for efficient ecological control and management of this valuable fisheries resource.

• 한국약용작물학회지
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• 제23권6호
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• pp.439-445
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• 2015

Background : Correct identification of Panax species is important to ensure food quality, safety, authenticity and health for consumers. This paper describes a high resolution melting (HRM) analysis based method using internal transcribed spacer (ITS) and 5.8S ribosomal DNA barcoding regions as target (Bar-HRM) to obtain barcoding information for the major Panax species and to identify the origin of ginseng plant. Methods and Results : A PCR-based approach, Bar-HRM was developed to discriminate among Panax species. In this study, the ITS1, ITS2, and 5.8S rDNA genes were targeted for testing, since these have been identified as suitable genes for use in the identification of Panax species. The HRM analysis generated cluster patterns that were specific and sensitive enough to detect small sequence differences among the tested Panax species. Conclusion : The results of this study show that the HRM curve analysis of the ITS regions and 5.8S rDNA sequences is a simple, quick, and reproducible method. It can simultaneously identify three Panax species and screen for variants. Thus, ITS1HRM and 5.8SHRM primer sets can be used to distinguish among Panax species.

• 생명과학회지
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• 제33권11호
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• pp.897-904
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• 2023

본 연구는 Bacillus velezensis K10의 유전체 분석결과에 따른 유전자의 고유한 특성을 이용하여 유전자마커를 탐색하고 확립하여 산업현장에서 활용하기 위해서 수행하였다. B. velezensis K10은 총 4,159,835 bps를 유지하였으며, 5,136개의 단백질을 발현하는 것으로 조사되었다. B. velezensis K10은 표준균주에 비교하여 전반적으로 외부요인에 기인되는 유전자의 이동이 훨씬 많은 것으로 나타났다. 이와 같은 양상에 기인하여 B. velezensis K10은 특유의 유전적 서열을 유지할 수 있는 것으로 추정되었다. 선발마커 발굴을 위해 recombinase, integrase, transposase, phage-related genes, 등 유전자 변이 유발이 쉬운 게놈상의 영역에 대해 탐색을 실시하였다. 그 결과, 선발마커로써 가능성이 높은 9개 부위를 확보하였다. 후보마커는 일부 다른 영역에서 특이성을 보이는 영역들이 존재했지만, phage 연관 유전자들에서 매우 특이성이 높았기 때문에, 모두 phage 관련 부위에서 모두 탐색되었다. 종간 후보 선발마커로써 B. licheniformis K12, B. velezensis K10, B. subtilis, B. cereus 등에 대해 PCR 분석을 실시하였다. 그 결과 BV3, BV5~9까지 총 6 프라이머 세트에서 B. velezensis K10 특이적인 PCR 산물이 형성되는 것을 확인하였다. 다른 한편으로, subspecies 수준에서 분석 결과, BV3, 5, 8, 9 등 4 프라이머 세트에서 B. velezensis K10 특이적인 PCR 산물이 형성되는 것을 관찰했다. 분석된 마커 중에서 BV5와 8가 가장 특이성이 높았기 때문에 종(species) 및 아종(sub-species) 수준에서 B. velezensis K10 유전자 선발마커로써 BV5와 8을 활용 가능할 것으로 제의된다.

• Journal of Microbiology and Biotechnology
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• 제25권11호
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• pp.1928-1935
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• 2015

Microbial growth kinetics is often used to optimize environmental processes owing to its relation to the breakdown of substrate (contaminants). However, the quantification of bacterial populations in the environment is difficult owing to the challenges of monitoring a specific bacterial population within a diverse microbial community. Conventional methods are unable to detect and quantify the growth of individual strains separately in the mixed culture reactor. This work describes a novel quantitative PCR (qPCR)-based genomic approach to quantify each species in mixed culture and interpret its growth kinetics in the mixed system. Batch experiments were performed for both single and dual cultures of Pseudomonas putida and Escherichia coli K12 to obtain Monod kinetic parameters (μ_max and K_s). The growth curves and kinetics obtained by conventional methods (i.e., dry weight measurement and absorbance reading) were compared with that obtained by qPCR assay. We anticipate that the adoption of this qPCR-based genomic assay can contribute significantly to traditional microbial kinetics, modeling practice, and the operation of bioreactors, where handling of complex mixed cultures is required.

• Parasites, Hosts and Diseases
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• 제51권1호
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• pp.1-8
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• 2013

Taenia solium, T. saginata, and T. asiatica are taeniid tapeworms that cause taeniasis in humans and cysticercosis in intermediate host animals. Taeniases remain an important public health concerns in the world. Molecular diagnostic methods using PCR assays have been developed for rapid and accurate detection of human infecting taeniid tapeworms, including the use of sequence-specific DNA probes, PCR-RFLP, and multiplex PCR. More recently, DNA diagnosis using PCR based on histopathological specimens such as 10% formalin-fixed paraffin-embedded and stained sections mounted on slides has been applied to cestode infections. The mitochondrial gene sequence is believed to be a very useful molecular marker for not only studying evolutionary relationships among distantly related taxa, but also for investigating the phylo-biogeography of closely related species. The complete sequence of the human Taenia tapeworms mitochondrial genomes were determined, and its organization and structure were compared to other human-tropic Taenia tapeworms for which complete mitochondrial sequence data were available. The multiplex PCR assay with the Ta4978F, Ts5058F, Tso7421F, and Rev7915 primers will be useful for differential diagnosis, molecular characterization, and epidemiological surveys of human Taenia tapeworms.

• 산업식품공학
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• 제21권2호
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• pp.174-179
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• 2017

For preliminary molecular typing, PCR-based fingerprinting using random amplified polymorphic DNA (RAPD) is the method of choice. In this study, 14 bacterial strains were isolated from different Korean food sources, identified using 16S rRNA gene sequencing, and characterized through RAPD-PCR. Two PCR primers (239 and KAY3) generated a total of 130 RAPD bands, 14 distinct PCR profiles, 10 polymorphic bands, one monomorphic band, and four unique bands. Dendrogram-based analysis with primer 239 showed that all 14 strains could be divided into seven clades out of which clade VII had the maximum of seven. In contrast, dendrogram analysis with the primer KAY3 divided the 14 L. citreum strains into four clades out of which clade IV consisted of a maximum of 10 strains out of 14. This research identified and characterized bacterial populations associated with different Korean foods. The proposed RAPD-PCR method, based on sequence amplification, could easily identify and discriminate the lactic acid bacteria species at the strain-specific level and could be used as a highly reliable genomic fingerprinting tool.