Buffalo specific primer, kit and application thereof in buffalo origin component identification
A source-derived component and specific technology, applied in the determination/inspection of microorganisms, biochemical equipment and methods, DNA/RNA fragments, etc., can solve problems that have not been studied in other species, and achieve low cost, wide applicability, highly specific effect
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Embodiment 1
[0033] Specific detection of buffalo-derived components in the sample of Example 1
[0034] 1. Sample preparation and storage
[0035] 1.1 Sampling
[0036] Collect 1 g of buffalo meat samples and store them at -20°C for future use.
[0037] 1.2 DNA template preparation
[0038] The DNA template was prepared using the commonly used phenol-chloroform crude extraction method (Sambrook J, Fritsch EF, Maniartis T. Molecular Cloning Experiment Guide [M]. 2nd Edition. Jin Dongyan, Li Mengfeng. Beijing: Science Publishing Society, 1999.465-467) or recognized other extraction methods with the same efficacy, these methods are the commonly used methods reported.
[0039] 2. Primer Design
[0040] The primer sequences of this embodiment are shown in Table 2 and SEQ ID NO: 2 and 3 in the sequence listing.
[0041] Table 2 PCR amplification primers designed by the present invention
[0042]
[0043]
[0044] The size of the expected amplified fragment is 231bp, and its nucleoti...
Embodiment 2
[0066] Embodiment 2 sensitivity test
[0067] Using 0.1ng / μL, 1ng / μL, 10ng / μL, and 100ng / μL buffalo DNA as templates, the nucleotide-specific fragment of SEQ ID NO.1 was amplified according to the conditions of Example 1. The result is as figure 2 As shown, there is amplification at a template concentration of 1ng / μL, indicating that the fragment amplified by the specific primer has good sensitivity.
Embodiment 3
[0068] The assembly of embodiment 3 kits
[0069] The kit consists of:
[0070] Upstream primer (SEQ ID No.2);
[0071] Downstream primer (SEQ ID No.3);
[0072] 2×Taq DNA Master Mix;
[0073] Positive control DNA template (buffalo DNA template);
[0074] double distilled water.
[0075] Storage of this kit at -20°C for 12 months will not affect the use effect.
[0076] How to use the kit:
[0077] 1. Load the sample into a 200 μL EP tube according to the following PCR reaction system:
[0078]
[0079] 2×TaqDNAMasterMix (purchased from Beijing Aidelai Biotechnology Co., Ltd.) is the Taq enzyme, dNTP mixture, MgCl 2 And the reaction buffer is pre-configured into a 2-fold concentration mixture.
[0080] 2. Loading according to the PCR amplification conditions of Example 1
[0081] 3. After the reaction, take 5 μL of the PCR amplification product, electrophoresis on a 2.0% agarose gel (technical parameters: 2V / cm~5V / cm, electrophoresis 15min~30min), stain with ethidi...
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