Specific primers and liquid chip kit for xrcc1 gene mutation detection
A kit and detection solution technology, applied in the field of molecular biology, can solve problems such as the use of antibodies and the judgment of operation steps without uniform standards, affecting promotion and application, and detection limitations, so as to achieve consistent detection results, simple steps, and avoid crossover The effect of the reaction
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Embodiment 1
[0025] The XRCC1 gene mutation detection liquid chip kit described in this embodiment mainly includes:
[0026] 1. ASPE Primers
[0027] Specific primer sequences were designed for the wild-type and mutant types of the three common genotypes A1196G, C580T and G839A of the XRCC1 gene. ASPE primers consist of "tag sequence + specific primer sequence". ASPE primer sequences are shown in the table below:
[0028] Table 1 ASPE primer sequence (tag sequence + specific primer sequence) of XRCC1 gene
[0029]
[0030] Each ASPE primer includes two parts, the 5' end is a specific tag sequence for the anti-tag sequence on the corresponding microsphere, and the 3' end is a mutant or wild-type specific primer fragment (as shown in the above table 1). Among them, the bases marked in the "box" were used as the target to detect the wild-type and mutant bases of the mutation site, and all ASPE primers were synthesized by Shanghai Sangon Bioengineering Technology Service Co., Ltd. Each ...
Embodiment 2
[0042] Example 2 Detection of samples using the XRCC1 gene mutation detection liquid chip kit described in Example 1
[0043] The formula of described various solutions is as follows:
[0044] 50mM MES buffer (pH5.0) formula (250ml):
[0045]
[0046] 2×Tm hybridization buffer
[0047]
[0048] Store at 4°C after filtration.
[0049] ExoSAP-IT kit was purchased from US USB Company.
[0050] Biotin-labeled dCTP was purchased from Shanghai Sangon Bioengineering Technology Service Co., Ltd.
[0051] 1. Sample DNA extraction:
[0052] Refer to the relevant methods of DNA extraction in "Molecular Cloning" to obtain the DNA to be detected.
[0053] 2. PCR amplification of samples to be tested
[0054] Design 3 pairs of primers and multiplex PCR to amplify 3 mutation sites containing three targets of the XRCC1 gene in one step
[0055] The target sequences of A1196G, C580T and G839A have product sizes of 312bp, 337bp and 312bp respectively, and the primer sequences (SEQ ...
Embodiment 3
[0098] Example 3 Detection of the SNP site of the XRCC1 gene by the liquid chip kit with different ASPE primers
[0099] 1. Design of liquid phase chip preparation (selection of Tag sequence and Anti-Tag sequence)
[0100] Taking the XRCC1 gene A1196G and G839A site mutation detection liquid chip as an example, the specific primer sequence of the 3' end of the ASPE primer was designed for the wild type and mutant type of A1196G and G839A, and the Tag sequence at the 5' end of the ASPE primer was selected from SEQ ID NO.1-SEQ ID NO.6, correspondingly, the anti-tag sequence coated on the microsphere and complementary to the corresponding tag sequence is selected from SEQ ID NO.13-SEQ ID NO.18. The specific design is shown in the following table (Table 7). The synthesis of ASPE primers, microspheres coated with anti-tag sequences, amplification primers, detection methods, etc. are as described in Example 1 and Example 2.
[0101] Table 7 Design of liquid phase chip preparation ...
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