Construction of pig peripheral bloodmononuclear lymphocytePD-L1 (programmed death-ligand1) recombinantplasmids, real-time gene abundance detection method and application of method
A PD-L1, peripheral blood single technology, applied in the field of molecular pathology and immunology, to achieve the effect of simple operation, high detection throughput and high sensitivity
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Embodiment 1
[0043] Example 1 Construction of porcine PD-L1 real-time fluorescence quantitative PCR positive standard recombinant plasmid
[0044] The peripheral blood of 45-day-old piglets was collected, and the lymphocytes in the peripheral blood were separated according to the instructions of the lymphocyte separation medium, and the total RNA was extracted according to the instructions of the Invitrogen TRIzol kit and related literature. The extracted total RNA was reverse-transcribed into cDNA according to the instructions of the reverse transcription kit, and stored at -20°C for use as a template for amplifying the target gene fragment of PD-L1.
[0045] The target gene fragment of PD-L1 is amplified by ordinary PCR method, and the target gene fragment is detected by agarose gel electrophoresis, recovered and purified; then the purified fragment of the PD-L1 target gene is connected to the pMD 18-T vector, and transformed into a Extract the recombinant plasmid from DH5α cells in st...
Embodiment 2
[0056] Example 2: Establishment of porcine PD-L1 real-time fluorescent quantitative PCR system
[0057] (1) Preparation of plasmid DNA template
[0058] The target gene fragment of PD-L1 was amplified by ordinary PCR amplification method, and the target gene fragment was detected by 2% agarose gel electrophoresis, recovered and purified, and transformed into competent cells after ligation with pMD 18-T vector (TaKaRa, Dalian) In DH5α, the recombinant plasmid was extracted; after clone screening, sequencing analysis was performed, and the sequencing results showed that it was 100% homologous to the sequence of the porcine PD-L1 gene in GenBank, indicating that the obtained sequence was correct, and the positive plasmid could be used for the production of plasmid standards. The standard plasmid DNA concentration was determined to be 300 μg / mL using a micronucleic acid protein spectrophotometer, and the initial standard plasmid solution was diluted 1:10 times.
[0059] (2) Cal...
Embodiment 3
[0073] Example 3 : Sensitivity, specificity and repeatability analysis of porcine PD-L1 real-time fluorescent quantitative PCR system
[0074] The porcine PD-L1 recombinant plasmid constructed in Example 1 was used as the positive recombinant standard plasmid; the porcine PD-L1 real-time fluorescent quantitative PCR detection system established in Example 2 was used; the real-time fluorescent quantitative PCR instrument was produced by Life Technologies (USA) ABI 7500 fluorescent quantitative PCR instrument was used.
[0075] with 10-fold serial dilutions of 10 1 ~10 9 The copies / μL porcine PD-L1 positive recombinant standard plasmid was used for the sensitivity test, and the results showed that the detection limit of PD-L1 was 10 copies / μL.
[0076] Real-time-PCR melting curve for porcine PD-L1 molecule (see attached Figure 4 ) and product agarose gel electrophoresis for specificity analysis, the results showed that a single narrow peak appeared in the melting curve, a...
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