Special primer for double PCR of contagious pustular dermatitis virus and mycoplasma ovipneumoniae

A technology for mycoplasma pneumoniae and impetigo virus, applied in the direction of microorganisms, recombinant DNA technology, and methods based on microorganisms, to achieve the effect of accurate diagnosis of pathogens

Active Publication Date: 2017-05-10
INST OF ANIMAL HUSBANDRY & VETERINARY FUJIAN ACADEMY OF AGRI SCI
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

Some scholars at home and abroad have used PCR technology to diagnose and epidemiologically study sheep contagious impetigo and goat contagious pleuropneumonia. In China, Qu Yonggang et al., Li Yuan et al., and Chu Yuefeng et al. respectively established PCR detection methods for ovine mycoplasma pneumoniae. and Mycoplasma ovis pneumonia...

Method used

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  • Special primer for double PCR of contagious pustular dermatitis virus and mycoplasma ovipneumoniae
  • Special primer for double PCR of contagious pustular dermatitis virus and mycoplasma ovipneumoniae
  • Special primer for double PCR of contagious pustular dermatitis virus and mycoplasma ovipneumoniae

Examples

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Comparison scheme
Effect test

Embodiment 1

[0025] Example 1 The design of the special primer B2L for the rapid detection of sheep infectious pustulosis virus of the present invention and the detection of sheep infectious pustulosis virus using the pair of special primers B2L using a single PCR method.

[0026] (1) Design and synthesis of the special primer B2L for detecting sheep infectious pustular virus

[0027] The special primer B2L for detecting sheep infectious pustulosis virus is based on the B2L gene segment in the sheep infectious pustulus virus genome, using Primer 6.0 primer design software to design specific primers, and number them as special primer B2L, which is composed of special primers B2L ​​upstream primer and dedicated primer B2L downstream primer, the base sequence of the dedicated primer B2L upstream primer is 5'-AGGCGGGCGTCAACTACTACAA-3', and the base sequence of the dedicated primer B2L downstream primer is 5'-TTCTTGGCGTTCTCGATGCGGT-3' The target product fragment length of the special primer B2L for ...

Embodiment 2

[0044] Example 2 The design of the special primer P80 for rapid detection of Mycoplasma ovipneumoniae of the present invention and the use of the pair of special primers P80 to detect Mycoplasma ovipneumoniae by a single PCR method.

[0045] (1) Design and synthesis of the special primer P80 for detecting Mycoplasma ovis pneumoniae

[0046] The special primer P80 for detection of Mycoplasma ovis pneumoniae is based on the P80 gene fragment of Mycoplasma ovis pneumoniae, using Primer 6.0 primer design software to design a specific primer, and number it as the special primer P80, which is composed of the special primer P80 upstream primer and the special primer P80 The downstream primer is composed of the base sequence of the upstream primer of the dedicated primer P80 is 5'-GCCTTGGGGTTGGAATTCCTTTGTCTTATTC-3', and the base sequence of the downstream primer of the dedicated primer P80 is 5'-CATTTGATGCTGAGGTCGGATTTGGACTAAC-3', and the detection The target product fragment length of the...

Embodiment 3

[0051] Example 3 Double PCR specificity test of sheep infectious pustular virus and Mycoplasma ovis pneumoniae

[0052] (1) PCR reaction of mixed template samples.

[0053] Using sheep infectious pustulum virus DNA, mycoplasma ovis pneumoniae DNA and a mixed sample of sheep infectious pustular virus DNA and Mycoplasma ovis pneumoniae DNA as templates, using Mycoplasma ovis pneumoniae DNA, Mycoplasma mycoplasma goat subspecies DNA, and parapig hematopoietic DNA Bacillus coli DNA, Escherichia coli DNA, Laiye Cholesterogen DNA, Staphylococcus aureus DNA, Pasteurella multocida DNA, Mycoplasma capricolum subsp. goat pneumonia DNA were negative controls, and deionized water was used as a blank control. The sample templates were respectively amplified by PCR using the optimal reaction system of the present invention described in Table 2.

[0054] The optimal reaction system of the present invention described in Table 2 performs PCR amplification

[0055]

[0056] The reaction conditions are...

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Abstract

The invention provides a special primer for double PCR of a contagious pustular dermatitis virus and mycoplasma ovipneumoniae. According to the special primer, two pairs of specific primers capable of amplifying a B2L gene and a P80 gene are designed according to the B2L gene of the contagious pustular dermatitis virus and the P80 gene of the mycoplasma ovipneumoniae. Through optimization of the conditions of the primer concentration, the annealing temperature and the like, a double PCR method for fast detecting the contagious pustular dermatitis virus and the mycoplasma ovipneumoniae is built. A specific segment of 401bp appearing in an electrophoretogram has positive contagious pustular dermatitis virus, and the specific segment of 700bp has positive mycoplasma ovipneumoniae. Detection of the contagious pustular dermatitis virus and the mycoplasma ovipneumoniae in the same reaction system can be achieved, the special primer has the advantage that the pathogens are fast, specifically and accurately diagnosed, and a novel method is provided for differential diagnosis of infection of the two pathogens in production and epidemiological investigation.

Description

Technical field [0001] The invention relates to a special primer for double PCR of sheep infectious pustular virus and Mycoplasma ovis pneumoniae and a double PCR detection method, belonging to the field of preventive veterinary medicine. Background technique [0002] Contagious ecthyma (CE), commonly known as sheep aphthous (Orf), is an acute, contact and addictive disease of goats, sheep and humans caused by Orf virus (ORFV) infection. Epithelial zoonotic disease. The incidence of the disease is 4%-100%, and the mortality rate is 1%-59%. Mycoplasma ovipneumoniae (Mo) is one of the main pathogens that cause Mycoplasma pneumonia in sheep and goats. The clinical symptoms of Mycoplasma pneumonia are high fever, cough, gasping, progressive weight loss, serous and fibrinous inflammation of lung and pleura. The incidence rate is 20%-60%, the case fatality rate is generally 30%-50%, and some are as high as 80%. Mo has a complex structure and difficult cultivation. There is still a l...

Claims

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Application Information

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IPC IPC(8): C12Q1/70C12Q1/68C12Q1/04C12N15/11C12R1/93C12R1/35
CPCC12Q1/686C12Q1/689C12Q1/701C12Q2600/16C12Q2537/143C12Q2565/125
Inventor 林裕胜胡奇林江锦秀游伟
Owner INST OF ANIMAL HUSBANDRY & VETERINARY FUJIAN ACADEMY OF AGRI SCI
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