• 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.

• Food Science and Biotechnology
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• 제18권5호
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• pp.1118-1123
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• 2009

Event-specific real-time polymerase chain reaction (PCR) detection method for genetically modified (GM) maize MIR604 was developed based on integration junction sequences between the host plant genome and the integrated transgene. In this study, 2 primer pairs and probes were designed for specific amplification of 100 and 111 bp DNA fragments from the zSSIIb gene (the maize endogenous reference gene) and MIR604. The quantitative method was validated using 3 certified reference materials (CRMs) with levels of 0.1, 1, and 10% MIR604. The method was also assayed with 14 different plants and other GM maize. No amplification signal was observed in real-time PCR assays with any of the species tested other than MIR604 maize. As a result, the bias from the true value and the relative deviation for MIR604 was within the range from 0 to 9%. Precision, expressed as relative standard deviation (RSD), varied from 2.7 to 10% for MIR604. Limits of detections (LODs) of qualitative and quantitative methods were all 0.1%. These results indicated that the event-specific quantitative PCR detection system for MIR604 is accurate and useful.

• Journal of Plant Biotechnology
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• 제42권3호
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• pp.196-203
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• 2015

2008년 이후 꾸준히 유전자변형생물체의 수입 승인이 증가하여 2015년 2월 기준 국내 131개의 이벤트가 식용, 사료용, 가공용으로 수입 및 유통 중이다. LMO의 비의도적 자연 생태계 유출을 파악하기 위해 선행되어야 하는 것은 명확한 LMO 도입유전자 검출 기법의 개발이며, 본 연구를 통해 2014년 7개 이벤트에 대한 도입유전자 검출 기법을 확립하였다. 현재까지 확보된 유전자 분석기법은 40개이며 이는 국내도입 LMO의 80%를 검출할 수 있는 과학적 근거를 제공할 것이다(Lee et al. 2015). LMO 자연환경 모니터링 및 사후관리 연구를 위해 단일이벤트를 검출할 수 있는 기법 연구는 앞으로 계속 수행할 계획이다.

• Journal of Microbiology and Biotechnology
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• 제17권2호
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• pp.335-341
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• 2007

For the development of qualitative and quantitative PCR methods of genetically modified (GM) pepper developed in Korea, a capsanthin-capsorubin synthase (CCS) gene was used as the endogenous reference gene. The primer pair ccs-F/R amplifying the pepper endogenous gene gave rise to an amplicon of 102 bp. No amplified product was observed when DNA samples from 16 different plants were used as templates. The construct-specific primer pairs amplifying the junction region of the bar gene and Ti7 introduced in GM pepper gave rise to an amplicon of 182 bp. Quantitative PCR assay was performed using a TaqMan probe and a standard plasmid as a reference molecule, which contained both an endogenous and event-specific sequence. For the validation of this method, the test samples containing 0.1, 1, 3, 5, and 10% GM pepper were quantified.

• 원예과학기술지
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• 제29권2호
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• pp.123-129
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• 2011

To identify unintended vertical gene-transfer rates from the developed transgenic plants, rapid and unequivocal techniques are needed to identify event-specific markers based on flanking sequences around the transgene and to distinguish zygosity such as homo- and hetero-zygosity. To facilitate evaluation of zygosity, a polymerase chain reaction technique was used to analyze a transgenic pepper line B20 (homozygote), P915 wild type (null zygote), and their F1 hybrids, which were used as transgene contaminated plants. First, we sequenced the 3'-flanking region of the T-DNA (1,277 bp) in the transgenic pepper event B20. Based on sequence information for the 3'- and 5'-flanking region of T-DNA provided in a previous study, a primer pair was designed to amplify full length T-DNA in B20. We successfully amplified the full length T-DNA containing 986 bp from the flanking regions of B20. In addition, a 1,040 bp PCR product, which was where the T-DNA was inserted, was amplified from P915. Finally, both full length T-DNA and the 1,040 bp fragment were simultaneously amplified in the F1 hybrids; P915 ${\times}$ B20, Pungchon ${\times}$ B20, Gumtap ${\times}$ B20. In the present study, we were able to identify zygosity among homozygous transgenic event B20, its wild type P915, and hemizygous F1 hybrids. Therefore, this novel zygosity identification technique, which is based on PCR, can be effectively used to examine gene flow for transgenic pepper event B20.

• Food Science and Biotechnology
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• 제18권3호
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• pp.694-699
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• 2009

A multiplex polymerase chain reaction (PCR) method was developed for the detection of 4 events of genetically modified (GM) soybean. The event-specific primers were designed from 4 events of GM soybean (RRS, A2704-12, DP356043-5, and MON89788). The lectin was used as an endogenous reference gene of soybean in the PCR detection. The primer pair YjLec-4-F/R producing 100 bp amplicon was used to amplify the lectin gene and no amplified product was observed in any of the 9 different plants used as templates. This multiplex PCR method allowed for the detection of event-specific targets in a genomic DNA mixture of up to 1% GM soybean mixture containing RRS, A2704-12, DP356043-5, and MON89788. In this study, 20 soybean products obtained from commercial food markets were analyzed by the multiplex PCR. As a result, 6 samples contained RRS. These results indicate that this multiplex PCR method could be a useful tool for monitoring GM soybean.

• Food Science and Biotechnology
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• 제17권4호
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• pp.829-832
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• 2008

A multiplex polymerase chain reaction (PCR) method was developed to simultaneously detect 4 varieties of genetically modified (GM) cotton. The event-specific primers were used to distinguish the 4 varieties of GM cotton (MON1445, MON15985, MON88913, and LLcotton25) using multiplex PCR. The acyl carrier protein 1 (Acp1) gene was used as an endogenous reference gene of cotton in the PCR detection. The primer pair Acp1-AF/AR containing a 99 bp amplicon was used to amplify the Acp1 gene and no amplified product was observed in any of the 13 different plants used as templates. This multiplex PCR method allowed for the detection of event-specific targets in a genomic DNA mixture of up to 1% GM cotton containing MON1445, MON15985, MON88913, and LLcotton25.

• Journal of Plant Biotechnology
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• 제42권2호
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• pp.117-122
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• 2015

캐놀라(canola)는 식용유 및 바이오 에너지 생산을 위해 전 세계적으로 널리 재배되는 작물이다. 캐놀라의 수요가 증가하면서 유전자변형 캐놀라에 대한 중요성이 높아짐에 따라 LM 캐놀라 재배면적이 해마다 증가하고 있다. 국내에서는 상업적으로 활용되는 캐놀라를 100% 전량 수입에 의존하고 있으며, 이에 따라 비의도적으로 유출 가능성이 있는 수입 LM 캐놀라의 안전관리 및 생태계 위해성 평가가 요구된다. 본 연구에서는 국내 수입 승인 유통 LM 캐놀라 5개 이벤트(Topas 19/2, Rf3, Ms8, RT73, T45)의 명확한 검출을 위한 동시증폭 검출법(multiplex PCR)을 확립하고자 하였다. PCR 반응 조건은 5개 LM 이벤트가 동시에 명확히 검출되는 최적 primer 농도 및 반응 조건을 통해 Topas 19/2 (95 bp), Rf3 (139 bp), Ms8 (250 bp), RT73 (317 bp), T45 (378 bp)의 서로 다른 생성물 크기로 명확히 구분되도록 하였다. 최적 primer 농도는 반응액 최종농도 0.3~1.0 pmol로 primer 쌍 마다 각각 다른 cocktail을 만들었고, PCR 반응 조건은 $95^{\circ}C$ 5분 반응 후, $95^{\circ}C$ 15초, $55^{\circ}C$ 20초 20회 반응하고, 다시 $95^{\circ}C$ 15초, $60^{\circ}C$ 20초 20 회 반응하였을 때 최적 검출이 이루어졌다. 본 연구의 결과로 제시된 multiplex PCR 검출 조건은 국내 수입 유통 LM 캐놀라의 자연환경 모니터링을 위한 검출에 있어 소요되는 연구인력, 비용 및 시간을 보다 효율적으로 개선할 수 있을 것으로 사료된다.

• Food Science and Biotechnology
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• 제17권3호
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• pp.569-572
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• 2008

A multiplex polymerase chain reaction (PCR) method was developed to simultaneously detect 3 events of genetically modified (GM) maize. The event-specific primers were used to discriminate the following 3 events of GM maize (DAS-59122-7, TC6275, and MIR604) using multiplex PCR method. The zein gene was used as an endogenous maize reference gene in the multiplex PCR detection. The primer pair Zein-FIR producing a 99 bp amplicon was used to amplify the zein gene. The primer JI-Das-F1/R1 for DAS-59122-7, JI-TC6275-F3/R3 for TC6275, and JI-MIR F1/R1 for MIR604 yielded an amplicon of 130, 162, and 197 bp, respectively. The detection limit of multiplex PCR was 1% for DAS-59122-7, TC6275, and MIR604 for one reaction.

• Journal of Plant Biotechnology
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• 제36권4호
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• pp.384-391
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• 2009

Previously, two events (H15 and B20) of transgenic pepper (Capsicum annuum L.) that enhanced resistance to Cucumber mosaic virus (CMV) by the introduction of CMV coat protein (CP) gene were constructed. Presently, a single copy number of the CP gene was revealed in H15 and B20 by Southern blot. To predict possible unintended effects due to transgene insertion in an endogenous gene, we carried out sequencing of the 5'-flanking region of the CP gene and a Blastbased search. The results revealed that insertion of the transgene into genes encoding putative proteins may occur in the H15 and B20 transgenic event. Mutiplex polymerase chain reaction (PCR) for simultaneous detection and identification of transgenic pepper was conducted with a set of nine primers. Both transgenic event were differentiated from non-transgenic event by the presence of 267 bp and 430 bp PCR products indicative of CP gene specific primer pairs and primer pairs targeting the CP gene and 35S promoter. H15 and B20 uniquely possessed a 390 bp and 596 bp PCR product, respectively. The presence of a 1115 bp product corresponding to intrinsic pepper actin gene confirmed the use of pepper DNA as the PCR template. The primer set and PCR conditions used presently may allow the accurate and simple identification of CMV resistant transgenic pepper.