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Cited 15 time in webofscience Cited 31 time in scopus
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Development of a Multiplex PCR Method to Detect Fungal Pathogens for Quarantine on Exported Cactiopen access

Authors
Choi, Hyun JiHong, Seong WonKim, Hyun-JuKwak, Youn-Sig
Issue Date
Feb-2016
Publisher
KOREAN SOC PLANT PATHOLOGY
Keywords
grafted cactus; PCR detection; quarantine pathogen
Citation
PLANT PATHOLOGY JOURNAL, v.32, no.1, pp 53 - 57
Pages
5
Indexed
SCIE
SCOPUS
KCI
Journal Title
PLANT PATHOLOGY JOURNAL
Volume
32
Number
1
Start Page
53
End Page
57
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/15700
DOI
10.5423/PPJ.NT.09.2015.0184
ISSN
1598-2254
2093-9280
Abstract
Major diseases in grafted cacti have been reported and Fusarium oxysporum, Bipolaris cactivora, Phytophthora spp. and Collectotrichum spp. are known as causal pathogens. These pathogens can lead to plant death after infection. Therefore, some European countries have quarantined imported cacti that are infected with specific fungal pathogens. Consequently, we developed PCR detection methods to identify four quarantined fungal pathogens and reduce export rejection rates of Korean grafted cacti. The pathogen specific primer sets F.oF-F.oR, B.CF-B.CR, P.nF-P.nR, and P.cF-P.CR were tested for F. oxysporum, B.cactivora, P. nicotinae, and P. cactorum, respectively. The F.oF-F.oR primer set was designed from the Fusarium ITS region; the B.CF-B.CR and P.nF-P.nR primers respectively from Bipolaris and Phytophthora ITS1; and the P.cF-P.CR primer set from the Ypt1protein gene region. The quarantine fungal pathogen primer pairs were amplified to the specific number of base pairs in each of the following fungal pathogens: 210-bp (F. oxysporum), 510-bp (B. cactivora), 313-bp (P. nicotinae), and 447-bp (P. cactorum). The detection limit for the mono- and multiplex PCR primer sets was 0.1 ng of template DNA under in vitro conditions. Therefore, each primer set successfully diagnosed contamination of quarantine pathogens in export grafted cacti. Consequently, our methodology is a viable tool to screen contamination of the fungal pathogen in exported grafted cacti.
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