Detection and quantification of Diaporthe destruens from soil using real-time PCR with a novel TaqMan probe

This study developed a TaqMan probe (TP) real-time polymerase chain reaction (qPCR) assay for the detection and quantification of Diaporthe destruens, the fungus causing sweet potato foot rot, in andosols. The primers and hybridization probe set were designed based on the ribosomal DNA internal tran...

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Published in	Soil Microorganisms Vol. 79; no. 1; pp. 57 - 63
Main Authors	Kawabe, Masato, Erika, Sato, Yoshida, Shigenobu, Sekiguchi, Hiroyuki
Format	Journal Article
Language	Japanese
Published	Japanese Society of Soil Microbiology 01.04.2025
Subjects	Diaporthe destruens Foot rot Real-time PCR Sweet potato TaqMan probe
Online Access	Get full text
ISSN	0912-2184 2189-6518
DOI	10.18946/jssm.79.1_57

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Abstract	This study developed a TaqMan probe (TP) real-time polymerase chain reaction (qPCR) assay for the detection and quantification of Diaporthe destruens, the fungus causing sweet potato foot rot, in andosols. The primers and hybridization probe set were designed based on the ribosomal DNA internal transcribed spacer region to specifically detect D. destruens DNA, but not the similar species Diaporthe batatas. The detection limit of the novel TP assay was verified to be 0.00005 ng DNA. Along a fungal density gradient created through artificial infestation of andosols, the TP assay showed that the greater D. destruens detectability compared to those of a qPCR assay based on SYBR Green (SG) staining. In natural andosols, the TP assay demonstrated 10-fold sensitive detection of fungal DNA than the SG assay in several samples. Thus, the newly developed TP assay is more suitable for the sensitive detection and quantification of D. destruens in andosols.
AbstractList	This study developed a TaqMan probe (TP) real-time polymerase chain reaction (qPCR) assay for the detection and quantification of Diaporthe destruens, the fungus causing sweet potato foot rot, in andosols. The primers and hybridization probe set were designed based on the ribosomal DNA internal transcribed spacer region to specifically detect D. destruens DNA, but not the similar species Diaporthe batatas. The detection limit of the novel TP assay was verified to be 0.00005 ng DNA. Along a fungal density gradient created through artificial infestation of andosols, the TP assay showed that the greater D. destruens detectability compared to those of a qPCR assay based on SYBR Green (SG) staining. In natural andosols, the TP assay demonstrated 10-fold sensitive detection of fungal DNA than the SG assay in several samples. Thus, the newly developed TP assay is more suitable for the sensitive detection and quantification of D. destruens in andosols.
Author	Kawabe, Masato Sekiguchi, Hiroyuki Erika, Sato Yoshida, Shigenobu
Author_xml	– sequence: 1 fullname: Kawabe, Masato organization: Division of Field Crop and Vegetable Research, Kyushu Okinawa Agricultural Research Center, NARO – sequence: 1 fullname: Erika, Sato organization: Division of Crop Pest Control Research, Institute for Plant Protection, NARO – sequence: 1 fullname: Yoshida, Shigenobu organization: Division of Crop Pest Control Research, Institute for Plant Protection, NARO – sequence: 1 fullname: Sekiguchi, Hiroyuki organization: Division of Crop Pest Control Research, Institute for Plant Protection, NARO
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SubjectTerms	Diaporthe destruens Foot rot Real-time PCR Sweet potato TaqMan probe
Title	Detection and quantification of Diaporthe destruens from soil using real-time PCR with a novel TaqMan probe
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