Primer set and application thereof for detecting koi herpesvirus sph gene
A koi herpes virus and primer set technology, applied in the biological field, can solve the problems of complex operation, low specificity and sensitivity, and achieve the effects of simple operation, improved specificity and sensitivity, and convenient identification
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Embodiment 1
[0077] Example 1 Screening of specific primer sets
[0078] Primer design:
[0079] According to the Sph gene of koi herpes virus (GenBank accession number AB375381.1), use PrimerExplorerV4 online software http: / / primerexplorer.jp / elamp4.0.0 / index.html to design and synthesize LAMP primers for detecting koi herpes virus: through Considering factors such as base composition, GC content, formation of secondary structure, Tm value, distance between primers, and stability of primer ends, etc., set and adjust the parameters of the primer design software, and design and synthesize 10 sets of primers for use in Screening for LAMP primers. Among the primers required by the LAMP method, the upstream external primer, downstream external primer, upstream internal primer and downstream internal primer are necessary, which directly determine the sensitivity and specificity of amplification. The 10 sets of primers synthesized in this example and the nucleotide sequences corresponding to e...
Embodiment 2
[0091] Example 2 Primer set detects SPH gene
[0092] (1) template:
[0093] Synthesis has the DNA molecule of nucleotide sequence shown in SEQ ID NO:41, and this DNA molecule is the gene sequence corresponding to koi herpes virus DNA polymerase gene (Sph gene) through individual nucleotide replacement, this DNA molecule Labeled as SPH, dilute the concentration of the resulting SPH DNA molecule to 85 ng / μL. Here, the reason for carrying out individual nucleotide substitutions in the Koi herpes virus Sph gene is to make it unable to be translated into an active functional protein to prevent environmental pollution.
[0094] (2) Amplification:
[0095] With the DNA molecule obtained in step (1) as a template, with the DNA molecule having the nucleotide sequence shown in SEQ ID NO:1 as the upstream external primer (i.e. FOP), having the nucleotide sequence shown in SEQ ID NO:2 The DNA molecule is the downstream external primer (i.e. BOP), the DNA molecule having the nucleotide...
Embodiment 3
[0103] Example 3 Primer set detects SPH gene
[0104] (1) template:
[0105] Same as the template in Example 2, that is, a DNA molecule having the nucleotide sequence shown in SEQ ID NO:46.
[0106] (2) Amplification:
[0107] With the DNA molecule obtained in step (1) as a template, with the DNA molecule having the nucleotide sequence shown in SEQ ID NO:1 as the upstream external primer (i.e. FOP), having the nucleotide sequence shown in SEQ ID NO:2 The DNA molecule is the downstream external primer (i.e. BOP), the DNA molecule having the nucleotide sequence shown in SEQ ID NO: 3 is the upstream internal primer (i.e. FIP), having the nucleotide sequence shown in SEQ ID NO: 4 The DNA molecule is the downstream internal primer (ie, BIP), and the amplification system is set, as shown in Table 4.
[0108] Table 4 LAMP reaction system (25 μL)
[0109] components
The final concentration in the reaction system
FIP
2.0μmol / L
BIP
2.0μmol / L
...
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