Preparation method of gene mutation and fusion gene positive reference
A technology that combines genes and reference products, applied in botany equipment and methods, biochemical equipment and methods, genetic engineering, etc., can solve problems that affect diagnosis and treatment, errors, and product quality that cannot meet safety and effectiveness
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Embodiment 1
[0036] Use PCDH lentivirus as a vector to prepare BRAF V600E gene mutation positive reference products:
[0037] (1) First, call out the genomic DNA sequence of the corresponding mutation site of the gene to be detected from the Genbank of the NCBI website, such as: BRAF V600E gene mutation, check the BRAF genomic DNA sequence surrounding the V600E mutation site, and 下游约500bp复制其序列,序列如下:ATCTATTAGTCCCTTTCAGACCTCTGACCTTGCTCAGTGGTAGTTGAGATATAACTGAAGACTCTAAATTATATAACAATGAGGTGAGAAAAACATAATATTTCTCTTCCCTAAGTGCAGACTAAGATACTATCTGCAGCATCTTCATTCCAATGAAGAGCCTTTACTGCTCGCCCAGGAGTGCCAAGAGAATATCTGGGCCTACATTGCTAAAATCTAATGGGAAAGTTTTAGGTTCTCCTATAAACTTAGGAAA GCATCTCACCTCATCCTAAC ACATTTCAAGCCCCAAAAATCTTAAAAGCAGGTTATATAGGCTAAATAGAACTAATCATTGTTTTAGACATACTTATTGACTCTAAGAGGAAAGATGAAGTACTATGTTTTAAAAGAATATTATATTACAGAATTATAGAAATTAGATCTCTTACCTAAACTCTTCATAATGCTTGCTCTGATAGGAAAATGAGATCTACTGTTTTCTTACTTACCGTTATCAGTTCAAGTTGAAAG T GAAATCTCGATGGAGTGGGTCCCATCAGTTTGAACAGTTGTCTGGATCCATTTTGTGGATGGTAAGAATTGAGGCTATTTTCCA...
Embodiment 2
[0067] Use the pMXs mimetic virus as a vector to prepare a positive reference product for BRAF gene mutation:
[0068] The pMXs retrovirus was used as the vector to carry out the same construction, the upstream and downstream primer restriction sites of BRAF should be changed, and the upstream primer sequence is: GGAATTCGCATCTCACCTCATCCTAAC;,
[0069] The downstream primer sequence is: CCCAAGCTTTAGTAACTCAGCAGCATCTCAG,
[0070] Among them, GAATTC and AAGCTT are EcoRI and HindIII enzyme cutting sites respectively, and the carrier and primer are digested with these two same enzymes, and then purified, ligated, heat shock transformed, extracted and identified recombinant plasmids, and site-directed rapid mutation And the subsequent preparation of virus packaging and the establishment of stable cell lines are all the same as the above-mentioned steps in Example 1.
Embodiment 3
[0072] Use PCDH lentivirus as a carrier to prepare a gene mutation-positive reference product for combined mutation of two genes of Kras and BRAF:
[0073] (1) Call out the genomic DNA sequence of the corresponding mutation site of the Kras gene to be detected from the Genbank of the NCBI website, the sequence is as follows:
[0074] CCGCAGAACAGCAGTCTGGCTATTTAGATAGAACAACTTGATTTTAAGATAAAAGAACTGTCTATGTAGCATTTATGCATTTTCTTAA GCGTCGATGGAGGAGTTTG TAAATGAAGTACAGTTCATTACGATACACGTCTGCAGTCAACTGGAATTTTCATGATTGAATTTTGTAAGGTATTTTGAAATAATTTTTCATATAAAGGTGAGTTTGTATTAAAAGGTACTGGTGGAGTATTTGATAGTGTATTAACCTTATGTGTGACATGTTCTAATATAGTCACATTTTCATTTTTTATTATAAGGCCTGCTGAAAATGACTGAATATAAACTTGTGGGTAG GGTGGC GTAGGCAAGAGTGCCTTGACGATACAGCTAATTCAGAATCATTTTGTGGACGAATATGATCCAACAATAGAGGTAAATCTTGTTTTAATATGCATATTACTGGTGCAGGACCATTCTTTGATACAGATAAAGGTTTCTCTGACCATTTTCATGAGTACTTATCAAGATAATTATGCTGAAAGTTAAGTTATCTGAAATGTACCTTGGGTTTCAAGTTATATGTTGAACTTATAT G AGTATGTCAGGGTCCATG ATGTTCACTCTCTGTGCATTTTGATTGGAAGTGTATTTCAGA...
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