Development of PCR Diagnosis System for Plant Quarantine Seed-borne Wheat Streak Mosaic Virus

Lee, Siwon; Kang, Eun-Ha; Chu, Yeon-Mee; Shin, Yong-Gil; Ahn, Tae‐Young

doi:10.7845/kjm.2013.3013

Cited by 21 publications

(27 citation statements)

References 26 publications

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“…및 종자전 염을 하고 Fribourg et al, 1977), 핵산은 3개의 단백질을 암호화하며 총 염기서열의 길이는 약 6.4 kb이다 (Koenig and Lesemann, 1981;Bernal et al, 2000). APLV는 파파리자, 비름과, 명아주과, 박과 및 가지과에서 감염 보고사례 (Gibbs and Harrison, 1969;Koenig and Bode, 1978 (Lee et al, 2013a;Lee et al, 2013c;Lee and Shin, 2014;Lee et al, 2014a;Lee et al, 2015)되어 바이러스 검역실적이 증가하였으나 (Shin, 2009;Lee et al, 2013b) 참 고 문 헌…”

Section: Andean Potato Latent Virus (Aplv)는 Group IV (+)unclassified

Development of PCR-base Diagnostic System for the Detection of Andean potato latent virus

Lee¹,

Kim²,

Kim³

et al. 2015

CNU Journal of Agricultural Science

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: Andean potato latent virus (APLV) is a phytopathogenic virus that belongs to the Group IV (+) sense ssRNA viruses of the genus Tymovirus. It mainly infects potatoes and is specified as a controlled quarantine virus in Korea. In this study, two primer sets of RT-PCR and nested PCR [set 2 (404 → 259 bp) and set 23 (501 → 349 bp)], were selected, which can rapidly and accurately diagnose APLV in quarantine sites. In addition, a modified-positive control plasmid is development, can possible verification of laboratory contamination in diagnosis of APLV detection. The PCR-base system developed in this study is expected to diagnose APLV and contribute to the plant quarantine in Korea.

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Section: Andean Potato Latent Virus (Aplv)는 Group IV (+)unclassified

Development of PCR-base Diagnostic System for the Detection of Andean potato latent virus

Lee¹,

Kim²,

Kim³

et al. 2015

CNU Journal of Agricultural Science

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“…Unfortunately the method is laden with issues of false positive reaction and low sensitivity (McGee, 1995;Caruso et al, 2003;Priou et al, 2006). As a result, molecular biological methods which are simpler and highly sensitive are at present the preferred choice in seed health testing procedures (Fonseca et al, 2005;Lee et al, 2013;Majumder et al, 2013;Munkvold, 2009;Park and Kim, 2004;Peiró et al, 2011).…”

Section: Serologymentioning

confidence: 99%

A mini-review on the development and emerging perspectives of seed pathology

Etebu¹,

Nwauzoma²

2017

Microbiol Res Int

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Seeds are the means of propagating about 90% of all food crops in the world, and they significantly influence yield potential in crop plants. Moreover, seeds are adversely affected by a number of factors such as postharvest and storage disease pathogens and unfavourable environmental conditions. Seed-borne pathogens represent a major threat to crop establishment and yield. Exposure of seeds to disease pathogens and other adverse conditions disrupts their normal physiology and metabolism which ultimately affects productivity. It is therefore imperative to promptly diagnose, treat, prevent and control seed related diseases. As with every other sphere of scientific studies, seed pathology has evolved tremendously over time; hence in this paper the development and emerging perspectives of this all important discipline was reviewed. Pathogen exclusion by detection and elimination of infested seed lots is required for disease management but traditional and conventional measures such as visual examination, use of media culture and serology are inadequate to detect pathogens associated with seed. In contrast, Nucleic acid-based molecular tools, such as the polymerase chain reaction (PCR) have emerged as faster and more reliable means for detecting and quantifying pathogens in seeds than conventional techniques.

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“…Second, when more than two kinds of viruses must be examined in the same seed, ELISA and PCR have to be applied separately, thereby wasting labor and manpower, and causing inconvenience in the quarantine site. Third, if the positive control sample group is not secured, PCR test errors and amplification or non-amplification are difficult to accurately assess [13]. Moreover, since the positive control group sample is infected with the virus, it may be difficult to distribute domestically and import [14].…”

mentioning

confidence: 99%

Development of PCR Diagnostic System for Detection of the Seed-Transmitted Tobacco Ringspot Virus in Quarantine

Lee

Choi

et al. 2015

Indian J Microbiol

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Tobacco ringspot virus (TRSV) is a plant quarantine virus in Korea. As such, a TRSV examination is conducted when importing various crops. In this study, RT-PCR and nested PCR systems for TRSV detection in quarantine sites, and the modified-positive control plasmid for proving laboratory contamination and false positive reactions were developed. The developed diagnostic system was used to detect TRSV in the quarantine site. It revealed that from 2012 to August 2014, a total of 12 cases were detected in imported various crops. The system is expected to continue contributing to TRSV detection in plant quarantine.

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Development of PCR Diagnosis System for Plant Quarantine Seed-borne Wheat Streak Mosaic Virus

Cited by 21 publications

References 26 publications

Development of PCR-base Diagnostic System for the Detection of Andean potato latent virus

Development of PCR-base Diagnostic System for the Detection of Andean potato latent virus

A mini-review on the development and emerging perspectives of seed pathology

Development of PCR Diagnostic System for Detection of the Seed-Transmitted Tobacco Ringspot Virus in Quarantine

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