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Identification methods of Liriomyza sativae, Liriomyza sativae and Liriomyza clover

A technology of Liriomyza sativa L. americana and Liriomyza sativa L. can be applied to the identification field of Liriomyza sativa L. americana, Liriomyza sativa L., and can solve the problems of heavy workload, poor repeatability, high requirements on experimental conditions and the like, Achieve the effects of stable sensitivity, simple operation and improved detection efficiency

Inactive Publication Date: 2016-03-09
INSPECTION & QUARANTINE TECH CENT OF GUANGDONG ENTRY EXIT INSPECTION & QUARANTINE BUREAU +1
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  • Description
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Problems solved by technology

Isoenzyme electrophoresis technology requires high professional skills of operators, and operators are required to be able to accurately interpret the electrophoretic zymogram; restriction fragment length polymorphism PCR technology can accurately distinguish related species of Liriomyza sativae, but the screening requirements are limited. The workload of the endonuclease species is relatively large; although random amplification polymorphic DNA PCR is simple to operate, the reproducibility is poor and the requirements for experimental conditions are relatively high.

Method used

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  • Identification methods of Liriomyza sativae, Liriomyza sativae and Liriomyza clover
  • Identification methods of Liriomyza sativae, Liriomyza sativae and Liriomyza clover

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Embodiment Construction

[0015] The specific primer identification method for Liriomyza sativae, Liriomyza sativae and Liriomyza trifolii of the present invention will be further described in detail below.

[0016] The identification method of Liriomyza sativae, Liriomyza sativae, and Liriomyza clover of the present invention is to synthesize respective specific primers respectively according to the mtDNA COI sequences of Liriomyza sativae, Liriomyza sativae, and Liriomyza clover, using the three The genomic DNA of Liriomyza sativae was used as a template, and three PCR amplifications using the same template but different primers were performed simultaneously to obtain respective PCR reaction products, and the respective PCR reaction products were taken for electrophoresis detection in agarose gel and electrophoresis buffer, and After staining, observe and image in the gel imaging system. At the same time, the amplified products are directly sequenced bidirectionally. The sequencing results are compare...

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Abstract

The invention discloses an identification method for Liriomyza sativae. To be specific, the identification method comprises the following steps: respectively synthetizing specific primers of L. sativae Blanchard, L. huidobrensis and L. trifolii according to mtDNA (mitochondrial deoxyribonucleic acid) COI sequences of the L. sativae Blanchard, the L. huidobrensis and the L. Trifolii; performing PCR (Polymerase Chain Reaction) amplification on genome DNA of the three Liriomyza sativae adopted as templates for three times under the condition of the same template but different primers, thereby obtaining PCR products of the three Liriomyza sativae; detecting, staining, observing and imaging the PCR product of each Liriomyza sativae; if a bright amplification belt is formed in an electrophoresis result of the PCR product of the specific primer of the L. sativae Blanchard and the molecular weight of the PCR product ranges from 250bp to 500bp, determining that the Liriomyza sativae with the PCR product is the L. sativae Blanchard; if a bright amplification belt is formed in an electrophoresis result of the PCR product of the specific primer of the L. sativae Blanchard, and the molecular weight of the PCR product ranges from 550bp to 600bp, determining that the Liriomyza sativae with the PCR product is the L. Huidobrensis; and if a bright amplification belt is formed in an electrophoresis result of the PCR product of the specific primer of the L. trifolii, and the molecular weight of the PCR product ranges from 450bp to 550bp, determining that the Liriomyza sativae with the PCR product is the L. Trifolii. The identification method is simple to operate, strong in repeatability and high in sensitivity and has the advantages of stability and rapidness.

Description

technical field [0001] The invention relates to an identification method of specific primers for Liriomyza sativae, specifically, an identification method for Liriomyza sativae, Liriomyza sativae and Liriomyza clover. Background technique [0002] L. sativae Blanchard, also known as vegetable leafminer, American melon leaflet, and alfalfa leaflet, was first discovered in Argentina in 1938 and is now distributed in 29 provinces, autonomous regions, and municipalities directly under the central government in my country, such as Hainan and Guangdong. , Fujian, Hubei, Hunan, Zhejiang, Anhui, Sichuan, Henan, Shandong, Beijing, etc. have caused serious harm to our country's fruits, vegetables, cotton, tobacco, flowers, etc., and have gradually become a prominent problem in the process of agricultural production in our country. question. The feeding habit of Liriomyza sativae is omnivorous, with a wide range of hosts, which can harm more than 110 kinds of vegetables and fruits in mo...

Claims

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Application Information

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Patent Type & Authority Patents(China)
IPC IPC(8): C12Q1/68
Inventor 吴佳教胡俊韬李志江顾渝娟刘海军李春苑胡学难
Owner INSPECTION & QUARANTINE TECH CENT OF GUANGDONG ENTRY EXIT INSPECTION & QUARANTINE BUREAU
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