Variant porcine reproductive and respiratory syndrome virus (PRRSV) TaqMan fluorescence quantitative RT-PCR detecting kit and application thereof

A technology for respiratory syndrome and detection kits, applied in fluorescence/phosphorescence, microbial determination/inspection, biochemical equipment and methods, etc., can solve problems such as incompatibility for rapid diagnosis, high requirements for disease materials, molecular contamination, etc.

Inactive Publication Date: 2010-06-16
INST OF ANIMAL HUSBANDRY & VETERINARY FUJIAN ACADEMY OF AGRI SCI +6
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

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Problems solved by technology

At present, there are many detection methods for reproductive and respiratory syndrome virus, such as virus isolation, in situ hybridization and RT-PCR technology, etc. Although virus isolation and in situ hybridization have high sensitivity, the operation is cumbersome and the cost is high. The cycle is long and the requirements for disease materials are high, so it is not suitable for the rapid diagnosis of clinical PRRSV; although the conventional RT-PCR detection method is convenient, fast and sensitive, RT-PCR requires electrophoresis and is prone to EB or molecular Contamination, and can not be carried out timing, quantitative monitoring, etc., and fluorescent quantitative RT-PCR method can overcome the above shortcomings, fluorescent quantitative PCR method is a new method introduced by the United States AppliedBiosystems in 1996, it by adding fluorescent groups in the PCR reaction, using Fluorescent signal accumulation monitors the entire PCR process in real time, and finally uses the standard curve to quantitatively analyze the unknown template. It not only realizes the leap from qualitative to quantitative PCR, but also has more timing, quantification and specificity than conventional PCR. Strong and effective solution to the PCR pollution problem, etc.

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  • Variant porcine reproductive and respiratory syndrome virus (PRRSV) TaqMan fluorescence quantitative RT-PCR detecting kit and application thereof
  • Variant porcine reproductive and respiratory syndrome virus (PRRSV) TaqMan fluorescence quantitative RT-PCR detecting kit and application thereof
  • Variant porcine reproductive and respiratory syndrome virus (PRRSV) TaqMan fluorescence quantitative RT-PCR detecting kit and application thereof

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Embodiment 1

[0103] The mutant porcine reproductive and respiratory syndrome virus TaqMan fluorescent quantitative RT-PCR detection kit of the present invention. It includes the following components: DEPC water, 5×AMV buffer, 2.5mM / L dNTP, 2.5umol / LMgcl 2 , 10xPCR Buffer, Nuclease Inhibitor, AMV reverse transcriptase, LA TaqDNA polymerase, Oligo(dT)18, 100nmol / L primer mixture, 10nmol / LTaqMan probe, positive plasmid standard, negative control (physiological saline),

[0104] (1) Upstream and downstream primer mixtures: According to the nsp2 sequence of PRRSV-VR2332, PRRSV-FJ04a, PRRSV-JXwn06 (EF641008.1) mutants provided by GenBank database, the plasmid was designed and constructed with PrimerExpress5.0 software and Oligo6.0 software A pair of primers and probes, UP Primer: 5'-AGCTGATGACACCTTTGAGT-3'LOW Primer: 5'-AGCCTCATATTCCGTCTGTG-3', the target fragment size is 125bp,

[0105] (2)TaqMan probe:

[0106] Fluorescent probe sequence 5’FAM-CCGCGTAGAACTGTGACAACAACGCT-TAMRA 3’

[0107] (3) Positive...

Embodiment 2

[0120] The application of the mutant porcine reproductive and respiratory syndrome virus TaqMan fluorescent quantitative RT-PCR detection kit of the present invention: (1). The DEPC water in the kit, 5×AMV buffer, 10×PCR Buffer, 2.5mmol / L dNTP, 2.5umol / L Mgcl 2 ,, Oligo(dT)18, 100nmol / L primer mixture, 10nmol / LTaqMan probe, dissolve at room temperature;

[0121] (2) Synthesize the primer mixture and probe,

[0122] (3) Establish a fluorescence quantitative PCR reaction system,

[0123] Fluorescence quantitative RT-PCR reaction system 25ul, 10xPCR Buffer 13.5ul, 2.5mM / L dNTP2.5ul, 100nmol / L upstream and downstream primers 0.8ul each, 10nmol / L probe 0.8ul, LA TaqDNA polymerase 2U, template 1.0ul , The rest is sterilized distilled water to make up to 25μl, the reaction conditions are 94℃ pre-denaturation 5min, then 94℃10s, 55℃20s, 70℃20s, a total of 45 cycles,

[0124] (4)Mg 2+ , Primer and probe concentration optimization

[0125] Take the plasmid standard as the test sample, and the Mg...

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Abstract

The invention discloses variant porcine reproductive and respiratory syndrome virus (PRRSV) TaqMan fluorescence quantitative RT-PCR detecting kit and application thereof. A primer and a TaqMan probe are designed and synthesized by referring to an NSP2 fragment gene sequence of the variant PRRSV and common PRRSV of a GenBank. By optimizing the reaction condition and constructing a standard plasmid product, a method for diagnosing the variant PRRSV by TaqMan fluorescence quantitative RT-PCR is established. A result indicates that the method has the advantages of strong specificity, high sensitivity, and the like and can detect the standard plasmid product with 264 copy numbers, and the virus quantity of 0.5623TICD50 is 10 times more sensitive than RT-PCR. By detecting 22 disease samples, 8 disease samples are positive, and the positive rate is 36.4 percent. Because the method has the advantages of quantification, high speed, accuracy, sensitivity, and the like, the invention is suitable for the diagnosis on the swinery infected variant PRRSV in the early stage, the medium stage and the later stage and plays an important role in effectively diagnosing, preventing and treating the highly pathogenic PRRSV.

Description

Technical field [0001] The invention relates to a variant porcine reproductive and respiratory syndrome virus TaqMan fluorescent quantitative RT-PCR detection device, in particular to a variant porcine reproductive and respiratory syndrome virus TaqMan fluorescent quantitative RT-PCR detection kit and application. Background technique [0002] Porcine reproductive and respiratory syndrome (PRRS) is a new infectious disease that appeared in the mid to late 1980s. It is caused by porcine reproductive and respiratory syndrome virus (PRRSV). Severe reproductive disorders such as abortion, premature delivery, stillbirth, and mummification of sows, and respiratory symptoms in piglets and fattening pigs. The disease first developed in the United States in 1987, and then quickly spread in Canada, European countries and Asia. Since the outbreak of this disease in my country at the end of 1995, it has become one of the main diseases that endanger the pig industry in my country. Since the ...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/70C12Q1/68G01N21/64C12R1/93
Inventor 周伦江王隆柏庄向生魏宏陈如敬车勇良
Owner INST OF ANIMAL HUSBANDRY & VETERINARY FUJIAN ACADEMY OF AGRI SCI
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