Species-specific primers in multiplex PCR for Bactrocera minax identification using an internal transcribed spacer

[Display omitted] •Immature stages of Bactrocera minax inside citrus can be identified within 2–3 h at the port of entry.•Seven pairs of species-specific primers were developed to prevent false positive or false negative identification of B. minax.•Multiplex PCR assay makes identification rapid, cos...

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Published inJournal of Asia-Pacific entomology Vol. 26; no. 4; pp. 102146 - 6
Main Authors Regmi, Prakriti, Tsai, Cheng-Lung, Lin, Ming-Ying, Chuang, Yi-Yuan, Yeh, Wen-Bin
Format Journal Article
LanguageEnglish
Published Elsevier B.V 01.12.2023
한국응용곤충학회
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Online AccessGet full text
ISSN1226-8615
1876-7990
DOI10.1016/j.aspen.2023.102146

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Abstract [Display omitted] •Immature stages of Bactrocera minax inside citrus can be identified within 2–3 h at the port of entry.•Seven pairs of species-specific primers were developed to prevent false positive or false negative identification of B. minax.•Multiplex PCR assay makes identification rapid, cost-effective, and more accurate. Bactrocera minax (Enderlein), commonly known as the Chinese citrus fly, is a citrus pest native to China and nearby countries. B. minax can cause substantial losses in citrus orchards. B. minax can be spread to countries free from it by the global trade of citrus and by travelers carrying citrus. Timely, convenient, and accurate identification of B. minax is essential in preventing its spread. In the present study, the nuclear ribosomal internal transcribed spacer 2 (ITS2) amplicon was used to design species-specific primer pairs that enable B. minax to be distinguished from 11 other fruit fly species. Four forward and four reverse species-specific primers were designed, and out of all possible sets of species-specific primer pairs obtained after intermixing them, seven sets of species-specific primer pairs were able to accurately identify B. minax. For B. minax identification, specific fragments ranging from 83 to 431 base pairs in length were amplified. The validity of the specific band only in B. minax was determined by visually inspecting the gel profile of the PCR product. B. minax was correctly identified using the designed species-specific primer pairs, with no cross-amplification with the 11 other fruit fly species included in the experiments. In addition to saving DNA sequencing costs, the application of these species-specific primer pairs facilitates rapid identification of B. minax, with identification in border scenarios being completable within 2–3 h.
AbstractList Bactrocera minax (Enderlein), commonly known as the Chinese citrus fly, is a citrus pest native to China and nearby countries. B. minax can cause substantial losses in citrus orchards. B. minax can be spread to countries free from it by the global trade of citrus and by travelers carrying citrus. Timely, convenient, and accurate identification of B. minax is essential in preventing its spread. In the present study, the nuclear ribosomal internal transcribed spacer 2 (ITS2) amplicon was used to design species-specific primer pairs that enable B. minax to be distinguished from 11 other fruit fly species. Four forward and four reverse species-specific primers were designed, and out of all possible sets of species-specific primer pairs obtained after intermixing them, seven sets of species-specific primer pairs were able to accurately identify B. minax. For B. minax identification, specific fragments ranging from 83 to 431 base pairs in length were amplified. The validity of the specific band only in B. minax was determined by visually inspecting the gel profile of the PCR product. B. minax was correctly identified using the designed species-specific primer pairs, with no cross-amplification with the 11 other fruit fly species included in the experiments. In addition to saving DNA sequencing costs, the application of these species-specific primer pairs facilitates rapid identification of B. minax, with identification in border scenarios being completable within 2–3 h.
[Display omitted] •Immature stages of Bactrocera minax inside citrus can be identified within 2–3 h at the port of entry.•Seven pairs of species-specific primers were developed to prevent false positive or false negative identification of B. minax.•Multiplex PCR assay makes identification rapid, cost-effective, and more accurate. Bactrocera minax (Enderlein), commonly known as the Chinese citrus fly, is a citrus pest native to China and nearby countries. B. minax can cause substantial losses in citrus orchards. B. minax can be spread to countries free from it by the global trade of citrus and by travelers carrying citrus. Timely, convenient, and accurate identification of B. minax is essential in preventing its spread. In the present study, the nuclear ribosomal internal transcribed spacer 2 (ITS2) amplicon was used to design species-specific primer pairs that enable B. minax to be distinguished from 11 other fruit fly species. Four forward and four reverse species-specific primers were designed, and out of all possible sets of species-specific primer pairs obtained after intermixing them, seven sets of species-specific primer pairs were able to accurately identify B. minax. For B. minax identification, specific fragments ranging from 83 to 431 base pairs in length were amplified. The validity of the specific band only in B. minax was determined by visually inspecting the gel profile of the PCR product. B. minax was correctly identified using the designed species-specific primer pairs, with no cross-amplification with the 11 other fruit fly species included in the experiments. In addition to saving DNA sequencing costs, the application of these species-specific primer pairs facilitates rapid identification of B. minax, with identification in border scenarios being completable within 2–3 h.
Bactrocera minax (Enderlein), commonly known as the Chinese citrus fly, is a citrus pest native to China and nearby countries. B. minax can cause substantial losses in citrus orchards. B. minax can be spread to countries free from it by the global trade of citrus and by travelers carrying citrus. Timely, convenient, and accurate identi fication of B. minax is essential in preventing its spread. In the present study, the nuclear ribosomal internal transcribed spacer 2 (ITS2) amplicon was used to design species-specific primer pairs that enable B. minax to be distinguished from 11 other fruit fly species. Four forward and four reverse species-specific primers were designed, and out of all possible sets of species-specific primer pairs obtained after intermixing them, seven sets of species-specific primer pairs were able to accurately identify B. minax. For B. minax identification, specific fragments ranging from 83 to 431 base pairs in length were amplified. The validity of the specific band only in B. minax was determined by visually inspecting the gel profile of the PCR product. B. minax was correctly identified using the designed species-specific primer pairs, with no cross-amplification with the 11 other fruit fly species included in the experiments. In addition to saving DNA sequencing costs, the application of these speciesspecific primer pairs facilitates rapid identification of B. minax, with identification in border scenarios being completable within 2–3 h. KCI Citation Count: 0
ArticleNumber 102146
Author Lin, Ming-Ying
Yeh, Wen-Bin
Regmi, Prakriti
Chuang, Yi-Yuan
Tsai, Cheng-Lung
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  surname: Regmi
  fullname: Regmi, Prakriti
  organization: Department of Entomology, National Chung Hsing University, 145 Xingda Rd., South Dist., Taichung City 402202, Taiwan, ROC
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  givenname: Cheng-Lung
  orcidid: 0000-0003-4319-686X
  surname: Tsai
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  organization: Department of Entomology, National Chung Hsing University, 145 Xingda Rd., South Dist., Taichung City 402202, Taiwan, ROC
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  givenname: Ming-Ying
  surname: Lin
  fullname: Lin, Ming-Ying
  organization: Department of Plant Medicine, National Chiayi University, 300 Syuefu Rd., Chiayi City 600355, Taiwan, ROC
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  givenname: Yi-Yuan
  surname: Chuang
  fullname: Chuang, Yi-Yuan
  organization: Department of Entomology, National Chung Hsing University, 145 Xingda Rd., South Dist., Taichung City 402202, Taiwan, ROC
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  givenname: Wen-Bin
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  fullname: Yeh, Wen-Bin
  email: wbyeh@nchu.edu.tw
  organization: Department of Entomology, National Chung Hsing University, 145 Xingda Rd., South Dist., Taichung City 402202, Taiwan, ROC
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Keywords Species-specific primers
Multiplex PCR
Bactrocera minax
Quarantine pest
Chinese citrus fly
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Snippet [Display omitted] •Immature stages of Bactrocera minax inside citrus can be identified within 2–3 h at the port of entry.•Seven pairs of species-specific...
Bactrocera minax (Enderlein), commonly known as the Chinese citrus fly, is a citrus pest native to China and nearby countries. B. minax can cause substantial...
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SubjectTerms Bactrocera
Bactrocera minax
China
Chinese citrus fly
Citrus
DNA
entomology
fruit flies
gels
internal transcribed spacers
international trade
Multiplex PCR
pests
polymerase chain reaction
Quarantine pest
species
Species-specific primers
농학
Title Species-specific primers in multiplex PCR for Bactrocera minax identification using an internal transcribed spacer
URI https://dx.doi.org/10.1016/j.aspen.2023.102146
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Volume 26
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