• 생명과학회지
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• 제18권3호
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• pp.374-380
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• 2008

본 연구는 무균성수막염 의심환자의 다양한 검체로부터 enterovirus의 진단을 위하여 real-time NASBA, 2 step RT-PCR 시험과 세포배양 시험을 각각 실시하여 각 시험법의 검출율, 특이도, 사용자 편리성, 시험소요 시간, 교차오염의 가능성 등을 비교 검토하였다. 비교시험 결과 전체 292건의 검체로부터 real-time NASBA에서 145건, 세포배양에서 101건, 2 step RT-PCR에서 86건이 양성으로 나타나 real-time NASBA가 가장 검출율이 높은 시험법임을 알 수 있었다. Enterovirus 외의 무균성수막염 원인바이러스에 대한 특이도 비교 시험결과 2 step RT-PCR 시험에서 rhinovirus 10건 중 1건이 위양성 반응을 나타내어 다른 시험법에 비해 특이도가 떨어지는 것으로 나타났다. Real-time NASBA는 하나의 튜브에서 증폭과 검출이 동시에 일어나 다른 시험과 비교하여 교차오염의 가능성이 낮으며 또한 시험 소요시간이 5시간 정도로 세포배양(5-14일 소요) 및 2 step RT-PCR(9시간소요) 에 비하여 신속하게 진단할 수 있어 일선병원이나 실험실에서 enterovirus를 검출을 위하여 적용할 수 있을 것으로 사료된다.

• 한국수의병리학회:학술대회논문집
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• 한국수의병리학회 2002년도 추계학술대회초록집
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• pp.139-139
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• 2002

돼지 설사유발 칼리시 바이러스(Porcine enteric calicivirus: PECV)도 자돈에서 설사를 일으키는 바이러스로 이미 알려졌다. RT-PCR과 nested PCR을 이용하여 국내 양돈장에서 PECV의 발생을 조사하고자 본 연구를 시도하였다. 설사 분변은 경기, 충남, 전북, 전남과 제주지역에 분포한 31개의 농장 102마리의 자돈에서 채취하여 의뢰된 것을 조사하였다. RT-PCR 과 nested PCR 을 위하여 RNA dependent RNA Polymerase (RDRP) 부위와 capsid 부위에서 각각 2 쌍의 primer를 작성하였다. RDRP 부위에서 RT-PCR을 시행했던 바, 3마리 (2.9％) 에서, nested PCR에서는 18마리 (17.6％)에서 양성반응이 나왔으며 capsid 부위에서 RT-PCR 결과 5마리 (4.9％), nested PCR에서는 18마리(17.6％)가 양성반응으로 확인되었다. 본 연구를 통하여 PECV가 국내에서 돼지 설사를 일으키는 주요 원인체 중 하나라는 것이 밝혀졌으며, nested PCR 기법이 돼지 설사분변에서 PECV를 검출하는 좋은 진단방법이었다.

• Journal of Plant Biology
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• 제38권3호
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• pp.267-274
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• 1995

Based upon the nucleotide sequence of As strain of cucumber mosaic virus (CMV-As0 RNA4, coat protein (CP) gene was selected for the design of oligonucleotide primers of polymerase chain reaction (PCR) for detection and identification of the virus. Reverse transcription and polymerase chain reaction (RT-PCR) was performed with a set of 18-mer CMV CP-specific primers to amplify a 671 bp fragment from crude nucleic acid extracts of virus-infected leaf tissues as well as purified viral RNAs. The minimum concentrations of template viral RNA and crude nucleic acids from infected tobacco tissue required to detect the virus were 1.0 fg and 1:65,536 (w/v), respectively. No PCR product was obtained when potato virus Y-VN RNA or extracts of healthy plants were used as templates in RT-PCR using the same primers. The RT-PCR detected CMV-Y strain as well as CMV-As strain. Restriction analysis of the two individual PCR amplified DNA fragments from CMV-As and CMV-Y strains showed distinct polymorphic patterns. PCR product from CMV-As has a single recognition site for EcoRI and EcoRV, respectively, and the product from CMV-Y has no site for EcoRI or EcoRV but only one site for HindIII. The RT-PCR was able to detect the virus in the tissues of infected pepper, tomato and Chinese cabbage plants.

• 식물조직배양학회지
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• 제25권6호
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• pp.519-524
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• 1998

한국산 수박 녹반 모자이크 바이러스(CGMMV-WK)를 TR-PCR 기술에 의해서 간편하고 확실한 진단방법을 구명하고 아울러 CGMMV의 외피단백질 유전자를 클로닝 하였다. 바이러스의 추출은 Lee등 (1996)의 간이 조즙액추출법을 변형하여 정제된 핵산 추출액을 사용하여도 RT-PCR이 양호하였으며, 20 pmol의 primer, reverse transcriptase (30 unit), Rnasin (5unit)이 첨가된 PCR 반응액에서 one step reaction으로 RT-PCR이 가능하였다. CGMMV의 진단을 위한 RT-PCR 조건으로 42$^{\circ}C$에서 45분간 cDNA를 합성하고 있어서 95$^{\circ}C$ 에서 2분간 per-denaturation하고 96$^{\circ}C$ 에서 30초, 6$0^{\circ}C$ 에서 30초 그리고 72$^{\circ}C$에서 1분간으로 36 cycle을 반응을 수행함으로서 간편하고 확실하게 CGMMV를 진단할 수 있었다. 또한 추출된 CGMMV의 외피단백질의 염기서열분석 한 결과 CGMMV-W와는 98.77%, CGMMV-SH와는 99.38%의 상동성을 가지고 있었으며 아미노산 서열은 모두 100%의 상동성을 가지고 있었다.

• The Plant Pathology Journal
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• 제16권1호
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• pp.48-51
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• 2000

Citrus tristeza virus (CTV) was identified form CTV-infected early satsuma mandarin (Citus unshiu) and yuzu (C.junos) by RT-PCR. The total RNAs were isolated from citrus bark and seaf tissues infected with CTV and reverse transcription was followed with primers designed for amplifying CTV coat protein gene. DNA fragments 738 bp were amplified by RT-PCR and these products were colned for sequence analysis. Based on the sequence analysis, this PCR product has 97% sequence homology to CTV (T-385) CP gene isolated from USA. RT-PCR assay for CTV detection was more sensitivity than ELISA assay which was done with anti-CTV CP antibody. This is the frist report about CTV identification in Cheju island Korea.

• Journal of Veterinary Science
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• 제21권5호
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• pp.71.1-71.10
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• 2020

Background: Feline calicivirus (FCV) is a major and highly infectious pathogen in cats worldwide. However, there have been limited studies about the status of FCV infections in Korea. Objectives: To investigate the current status of FCV infections in stray cats in Korea. Methods: A novel reverse transcription polymerase chain reaction (RT-PCR) assay was developed based on the conserved nucleotide sequences of reported FCV strains. Field swab samples were collected from 122 cats (2 hospital admitted cats and 120 stray cats) in 2016 and 2017. All the samples were tested by virus isolation and 2 different RT-PCRs, including the novel RT-PCR, for the detection of FCV. Results: The novel RT-PCR assay showed no cross-reactivity to the nucleic acids of the other feline pathogens tested, and the limit of detection was calculated as 10⁰ TCID₅₀/mL based on an in vitro assessment. The novel RT-PCR assay detected 5 positive samples from the 122 field samples, which showed perfect agreement with the results of the virus isolation method. In contrast, another RT-PCR assay used in a previous study in Korea detected no positive samples. The prevalence of FCV infection in stray cats was 2.5% (3/120) based on the results of virus isolation and the novel RT-PCR assays. Conclusions: The current study is the first report of the detection and prevalence of FCV in stray cats in Korea. The novel RT-PCR assay developed in this study showed high sensitivity and specificity, which indicates a useful diagnostic assay to identify FCV infection in cats.

• 식물병연구
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• 제23권4호
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• pp.363-366
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• 2017

최근 국내 맥류 재배지에서는 대부분 BaMMV, BaYMV, BYDV의 발생이 확인되고 있다. 본 연구에서는 multiplex reverse transcription polymerse chain reaction (mRT-PCR) 방법에 의해 이들 3종류의 바이러스를 동시에 진단하는 방법을 확립하였다. 이들 3종 바이러스의 외피단백질 유전자 정보를 활용하여 각 바이러스에 대한 primer를 제작하였다. mRT-PCR에 사용한 primer는 RT-PCR 반응의 민감도와 특이성에 의해 선발하여 primer 농도와 mRT-PCR의 조건을 설정하였다. 각 바이러스에 대하여 선발된 primer 사용에 의한 mRT-PCR 결과 BaMMV 594 bp, BaYMV 461 bp, BYDV 290 bp의 PCR 산물을 얻을 수 있었다. 본 연구에서 확립된 맥류 바이러스 동시진단방법은 신속하고 특이적인 진단 뿐 아니라 맥류 바이러스병의 전염 등 역학 연구에도 활용 될 것으로 기대된다.

• 대한의생명과학회지
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• 제22권4호
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• pp.215-219
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• 2016

The problems of tuberculosis and its drug resistance are very severe. Therefore, rapid and accurate drug susceptibility assay is required. Recently, there has been an increased understanding of the genetic mechanism of Mycobacterium tuberculosis (MTB) drug resistance as well as advancement of molecular technologies. While many gene mutations correlate well with drug resistance, many genes do not show a strong correlation with drug resistance. For this reason, the current study assessed the utility of rpoB mRNA as a target to detect live mycobacteria. In this study, RT-PCR targeting of rpoB mRNA in BCG treated with rifampin was performed. Conventional RT-PCR and real-time PCR targeting rpoB mRNA as well as 85B mRNA was performed to determine whether these two methods could distinguish between viable and non-viable MTB. The levels of rpoB and 85B mRNA detected by RT- PCR were compared in parallel with colony forming unit counts of BCG that were treated with rifampin for different periods of time. The data suggests that that even though both mRNA levels of rpoB and 85B decreased gradually when rifampin-treatment increased, the rpoB mRNA seemed to represent live bacteria better than 85B mRNA. This study clearly indicates that RT-PCR is a good method to monitor viable cell counts in the liquid culture treated with the anti-tuberculosis drug.

• Journal of Microbiology and Biotechnology
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• 제28권2호
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• pp.210-217
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• 2018

A one-step multiplex reverse transcription PCR (RT-PCR) method comprising six primer sets (for the detection of norovirus GI and GII, hepatitis A virus, rotavirus, and astrovirus) was developed to simultaneously detect four kinds of pathogenic viruses. The size of the PCR products for norovirus GI and GII, hepatitis A virus (VP3/VP1 and P2A regions), rotavirus, and astrovirus were 330, 164, 244, 198, 629, and 449 bp, respectively. The RT-PCR with the six primer sets showed specificity for the pathogenic viruses. The detection limit of the developed multiplex RT-PCR, as evaluated using serially diluted viral RNAs, was comparable to that of one-step single RT-PCR. Moreover, this multiplex RT-PCR was evaluated using food samples such as water, oysters, lettuce, and vegetable product. These food samples were artificially spiked with the four kinds of viruses in diverse combinations, and the spiked viruses in all food samples were detected successfully.

• 생태와환경
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• 제37권1호통권106호
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• pp.122-129
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• 2004

In an effort to develop the biomarker for monitoring the contamination of xenoestrogen in the freshwater environment of Korea, reverse transcription-polymerasechain reaction (RT-PCR) analysis of vitellogenin (VTG) gene expression was optimized in Hearisarsus Iaseo, Based on the homology of the VTG cDNA sequences between the common carp and zebra fish, a set of PCR primers for VTG mRNA amplification for H; labo was designed. VTG mRNA level in livers from female and male fishes was analyzed by RT-PCR following single injection of 17 beta estradiol($E_2$ 10 mg $kg^{-1}$ B.W.). As an internal control, beta actin mRNA was amplified. One us of total liver RNA was subjected to RT-PCR. In female the amount of PCR productof VfC gradually increased in the range from 16 to 34 cycles of amplification. On the contrary, in control male, PCR product first detected at 32 cycles of amplification and linearly increased up to 40 cycles of amplification. In $E_2$ injected male liver, the VTC mRNA level was similar to that in the female. Taken together, this result suggests that liver of male H. labo expresses minute amount of VTG mRNA which are2-l6 equivalent of female and that induction of VTG mRNA occurs in male liver after estrogen treatment. In conclusion, the optimized protocol for RT-PCR analysis of VTG mRNA expression in liver of male H. labo will provide the environmental monitoring method for the xenoestrogen contamination in the rivers in Korea.