Method for rapidly screening specific SNP (Single Nucleotide Polymorphism) probe based on quantum dot platform
The invention provides a method for rapidly screening specific SNP (Single Nucleotide Polymorphism) probes based on a quantum dot platform, which comprises the following steps: firstly, designing and synthesizing two forward NH2 modified probes (wild type and mutant type) and two reverse biotin modi...
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Format | Patent |
Language | Chinese English |
Published |
16.01.2024
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Abstract | The invention provides a method for rapidly screening specific SNP (Single Nucleotide Polymorphism) probes based on a quantum dot platform, which comprises the following steps: firstly, designing and synthesizing two forward NH2 modified probes (wild type and mutant type) and two reverse biotin modified oligonucleotides (wild type and mutant type); then the two probes are hybridized with wild oligonucleotides and mutant oligonucleotides respectively based on a quantum dot nucleic acid detection method, the specificity of the probes is determined, and the specific SNP probes can be obtained through rapid screening. The method disclosed by the invention is simple in design, the conventional synthesized long double-stranded DNA is used as a positive control, and the short single-stranded oligonucleotide only containing the SNP site is used as the positive control, so that the synthesis period and the synthesis cost are reduced; meanwhile, the steps of PCR amplification, denaturation before nucleic acid hybridiza |
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AbstractList | The invention provides a method for rapidly screening specific SNP (Single Nucleotide Polymorphism) probes based on a quantum dot platform, which comprises the following steps: firstly, designing and synthesizing two forward NH2 modified probes (wild type and mutant type) and two reverse biotin modified oligonucleotides (wild type and mutant type); then the two probes are hybridized with wild oligonucleotides and mutant oligonucleotides respectively based on a quantum dot nucleic acid detection method, the specificity of the probes is determined, and the specific SNP probes can be obtained through rapid screening. The method disclosed by the invention is simple in design, the conventional synthesized long double-stranded DNA is used as a positive control, and the short single-stranded oligonucleotide only containing the SNP site is used as the positive control, so that the synthesis period and the synthesis cost are reduced; meanwhile, the steps of PCR amplification, denaturation before nucleic acid hybridiza |
Author | QIU HUILIANG ZHOU NA ZHU HAITAO CHEN SIYI HUANG SINAN WANG HAILIN FANG MEIHONG |
Author_xml | – fullname: FANG MEIHONG – fullname: QIU HUILIANG – fullname: ZHOU NA – fullname: HUANG SINAN – fullname: CHEN SIYI – fullname: WANG HAILIN – fullname: ZHU HAITAO |
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DocumentTitleAlternate | 一种基于量子点平台快速筛选特异性SNP探针的方法 |
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Snippet | The invention provides a method for rapidly screening specific SNP (Single Nucleotide Polymorphism) probes based on a quantum dot platform, which comprises the... |
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SubjectTerms | BEER BIOCHEMISTRY CHEMISTRY COMPOSITIONS OR TEST PAPERS THEREFOR CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL ORENZYMOLOGICAL PROCESSES ENZYMOLOGY INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIRCHEMICAL OR PHYSICAL PROPERTIES MEASURING MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEICACIDS OR MICROORGANISMS METALLURGY MICROBIOLOGY MUTATION OR GENETIC ENGINEERING PHYSICS PROCESSES OF PREPARING SUCH COMPOSITIONS SPIRITS TESTING VINEGAR WINE |
Title | Method for rapidly screening specific SNP (Single Nucleotide Polymorphism) probe based on quantum dot platform |
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