• 한국식품위생안전성학회지
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• 제35권6호
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• pp.561-566
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• 2020

참돔은 등쪽에 푸른 반점이 흩어져 있고, 홍민어는 꼬리 쪽에 검은 점이 있어 원물 형태는 쉽게 구분할 수 있다. 그러나 횟감이나 필렛으로 이용 시 참돔과 홍민어를 구분하기 어려워, 참돔의 종 특이 primer를 개발 및 검증하고 모니터링을 통해 참돔의 위변조 사례를 조사하고자 하였다. 시료에서 gDNA를 추출하여 PCR을 진행하였으며 참돔 primer의 product size는 468 bp, 홍민어 primer의 product size는 181 bp으로 설계하였다. Multiplex PCR 결과 참돔과 홍민어에 대한 종 특이적 증폭이 확인되었다. 또한, 참돔과 홍민어 PCR 민감도 실험 결과 참돔 primer는 1 ng, 홍민어 primer는 0.1 ng 까지 밴드가 확인되었다. 모니터링 결과 참돔으로 구매한 시료 19건 모두 참돔으로 판정되었다. 따라서 본 연구에서 제작된 참돔과 홍민어 종에 대한 종 특이적 primer는 횟감 등 수산물에도 적용할 수 있어 현재 유통 및 판매되고 있는 참돔 및 홍민어 판별에 적합성을 확인하였다.

• 한국발생생물학회지:발생과생식
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• 제10권4호
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• pp.227-238
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• 2006

한반도의 동쪽에 위치해 있는 삼척(venus clam from Samcheok; VCS)과 원산(venus clam from Wonsan; VCW) 지역에서 채취된 민들조개(Gomphina aequilatera)에서 genomic DNAs(gDNAs)를 분리 추출하였다. 증폭산물은 primer agarose 전기영동법에 의해서 생성되었고, EtBr에 의해서 염색된 이후에 자외선에 의해서 확인되었다. 150 bp에서 2,400 bp에 해당되는 shared loci, polymorphic 및 specific loci를 얻기 위해서 BION-21, BION-23, BION-25, BION-27, BION-29, BION-31 및 BION-33와 같은 7개의 primer를 사용하였다. 본 연구에서 7개의 primer는 VCS 민들조개 집단에서 147개의 polymorphic loci(147/954 loci, 15.41%)와 VCW 집단에서 274개의 polymorphic loci(274/996 loci, 27.51%)를 확인하였다. 이것은 VCS 민들조개 집단에서 보다 VCW 집단에서 더 높은 유전적 변이를 나타내고 있다는 것을 제시하고 있다. 특히 BION-21 primer에 의해서 나타난 700 bp는 민들조개 2개 집단에서 공통적으로 확인되었으며, 이러한 것은 집단이나 종을 확인할 수 있는 marker로서 활용이 가능할 것이다. 이러한 특이한 primer는 개체, 종 및 집단에서 서로 다른 DNA 다형성을 나타내며, 개체나 집단을 확인하는 데 유용하다는 것을 알 수 있다. 2개 민들조개 집단의 개체들을 비교해 보았을 때 SAMCHEOK no. 03와 WONSAN no. 22에서 가장 긴 유전적 거리(0.696)를 나타내었다. 3개의 genetic groupings and dendrogram을 포함한 complete linkage cluster analysis을 통해서 볼 때 지리적 거리가 있었지만 삼척과 원산 2 민들조개 집단의 개체 정체성과 다소 가까운 친척관계를 확인시켜 주었다. 분자적인 표지인자로부터 얻어진 종내 분류와 clustering analyses은 패각 크기, 패각 형태 및 패각 색깔과 같은 형태적인 형질을 기초한 재래적인 종 분류를 지원하고 있다. 따라서 위에서 언급된 바와 같이 RAPD 분석은 VCS 민들조개 집단이 VCW 집단과 어느 정도 차이가 있다는 것을 확인시켜 주었다.

• The Plant Pathology Journal
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• 제34권6호
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• pp.490-498
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• 2018

Panicle blight and seed rot disease caused mainly by Burkholderia glumae and Burkholderia gladioli is threatening rice cultivation worldwide. The bacteria have been reported as seed-borne pathogens from rice. Accurate detection of both pathogens on the seeds is very important for limiting the disease dissemination. Novel primer pairs targeting specific molecular markers were developed for the robust detection of B. glumae and B. gladioli. The designed primers were specific in detecting the target species with no apparent cross-reactions with other related Burkholderia species at the expected product size. Both primer pairs displayed a high degree of sensitivity for detection of B. glumae and B. gladioli separately in monoplex PCR or simultaneously in duplex PCR from both extracted gDNA and directly preheated bacterial cell suspensions. Limit of detection was as low as 0.1 ng of gDNA of both species and $3.86{\times}10^2cells$ for B. glumae and $5.85{\times}10^2cells$ for B. gladioli. On inoculated rice seeds, the designed primers could separately or simultaneously detect B. glumae and B. gladioli with a detection limit as low as $1.86{\times}10^3cells$ per rice seed for B. glumae and $1.04{\times}10^4cells$ per rice seed of B. gladioli. The novel primers maybe valuable as a more sensitive, specific, and robust tool for the efficient simultaneous detection of B. glumae and B. gladioli on rice seeds, which is important in combating rice panicle blight and seed rot by early detection and confirmation of the dissemination of pathogen-free rice seeds.

• 한국식물병리학회지
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• 제14권1호
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• pp.92-98
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• 1998

RAPD analysis was performed from four host-specific toxin (HST) producing Alternaria, i.e., A. kikuchiana, A. mali, a. longipes and A. Longipes and A. alternata f. sp. lycopersici, nonpathogenic A. alternata and A. brassicicola to assess their phylogenetic relationship. DNA polymorphism was detected among species (pathotypes) of HST producing Alternaria by PCR amplification and differentiation of the species was recognized by RAPD analysis. Primer OPA-02 was the most profitable among 7 notificated primers for differentiation of the HST producing Alternaria species. UPGMA analysis of the RAPD bands from alternaria spp. revealed that HST producing Alternaria and nonpathogenic a. alternata are closely related.

• 대한수의학회지
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• 제45권2호
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• pp.199-205
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• 2005

DNA fingerprint patterns of 8 Brucella reference strains and 15 B. abortus field isolates were characterized by repetitive element sequence-based PCR (rep-PCR) using BOX- and ERIC-primers in this study. AMOS PCR differentiated all Brucella field isolates from B. abortus RB51, a vaccine strain by producing a B. abortus-specific 498 bp band. Rep-PCR using BOX-primer produced 13 to 18 bands with sizes of between 230 and 3,300 bp, and discriminated Brucella strains to the species level except B. canis and B. suis. PCR products amplified with ERIC primers were, however, not appropriate for differentiating the Brucella isolates. DNA fingerprint patterns for all B. abortus field isolates were identical among them and were put on one cluster with B. abortus biovar 1 reference strain in the dendrogram, indicating they were highly clonal. These results suggested that rep-PCR using BOX primer might to be a useful tool for calculating genetic relatedness among the Brucella species and for the study of brucellosis epidemiology.

• Molecules and Cells
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• 제23권2호
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• pp.220-227
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• 2007

The development of suitable genetic markers would be useful for defining species and delineating the species boundaries of morphologically indistinguishable sponges. In this study, genetic variation in the sequences of nuclear rDNA and the mitochondrial cytochrome c oxidase subunit 1 and 3 (CO1 and CO3) regions were compared in morphologically indistinguishable Korean Halichondriidae sponges in order to determine the most suitable species-specific molecular marker region. The maximal congeneric nucleotide divergences of Halichondriidae sponges in CO1 and CO3 are similar to those found among anthozoan cnidarians, but they are 2- to 8-fold lower than those found among genera of other triploblastic metazoans. Ribosomal internal transcribed spacer regions (ITS: ITS1 + ITS2) showed higher congeneric variation (17.28% in ITS1 and 10.29% in ITS2) than those of CO1 and CO3. Use of the guidelines for species thresholds suggested in the recent literature indicates that the mtDNA regions are not appropriate for use as species-specific DNA markers for the Halichondriidae sponges, whereas the rDNA ITS regions are suitable because ITS exhibits a low level of intraspecific variation and a relatively high level of interspecific variation. In addition, to test the reliability of the ITS regions for identifying Halichondriidae sponges by PCR, a species-specific multiplex PCR primer set was developed.

• Journal of Microbiology and Biotechnology
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• 제22권8호
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• pp.1113-1117
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• 2012

Shigella sonnei is a causal agent of fever, nausea, stomach cramps, vomiting, and diarrheal disease. The present study describes a quantitative polymerase chain reaction (qPCR) assay for the specific detection of S. sonnei using a primer pair based on the methylase gene for the amplification of a 325 bp DNA fragment. The qPCR primer set for the accurate diagnosis of Shigella sonnei was developed from publically available genome sequences. This quantitative PCR-based method will potentially simplify and facilitate the diagnosis of this pathogen and guide disease management.

• 대한의생명과학회지
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• 제10권4호
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• pp.333-339
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• 2004

A multiplex PCR assay targeting the yst and 16S rRNA genes of Yersinia enterocolitica was developed to specifically identify pathogenic Y. enterocolitica from pure culture. Simultaneous amplification of 145 and 416 bp fragments of the yst and 16S rRNA genes of Y. enterocolitica was obtained using the primer pairs in a single reaction. Validation of the assay was performed with the reference Yersinia strains and other members of the family Enterobacteriaceae. The defined primer pairs amplified the targeted sequence from only pathogenic Y. enterocolitica strains, whereas none of the other bacterial species yielded any amplified fragments. Within an assay time of 4 h, this assay offers a very specific, reliable, and inexpensive alternative to the conventional phenotypic assays used in clinical laboratories to identify pathogenic Y. enterocolitica.

• Journal of Microbiology and Biotechnology
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• 제23권4호
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• pp.555-559
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• 2013

Vibrio cholerae O1 and O139 are the major serotypes associated with illness, and some V. cholera non-O1 and non-O139 isolates produce cholera toxin. The present study describes a quantitative polymerase chain reaction (qPCR) assay for the species-specific detection and quantitation of V. cholera using a primer pair based on an outer membrane lipoprotein lolB gene for the amplification of a 195 bp DNA fragment. The qPCR primer set for the accurate diagnosis of V. cholera was developed from publically available genome sequences. This quantitative PCR-based method will potentially simplify and facilitate the diagnosis of this pathogen and guide disease management.

• 한국어병학회지
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• 제16권1호
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• pp.51-59
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• 2003

Streptococcal infection is one of the most serious disease of cultured olive flounder, Paralychthys olivaceus in Korea and caused by more than one species. However, there has been considerable confusions about the taxonomic position of the fish pathogenic streptococci. In this study, We performed the randomly amplified polymorphic DNA(RAPD) pattern analysis to evaluate the possible classification in 8 streptococci isolated from diseased olive flounder and reference strains based on their DNA structure. RAPD PCR with DNA solution prepared by simple boiling and 10-mer random primer was appeared to be a good tool for discrimination of different streptococcal strains. Phenotypical characters by simple biological test and API 20 Strep corresponded well to the specific profiles of RAPD in streptococcal isolates of this study. Therefore, the RAPD profile was considered as one of differential characters to discriminate the streptococcal isolates from diseased olive flounder.