Primer group, kit and method for detecting copy number of FRT sites in Flp-In host cell line
A host cell, flp-in technology, applied in the field of genetic engineering, can solve the problems of a large amount of genomic DNA, time-consuming, laborious, etc., and achieves the effects of good specificity, improved detection efficiency, and DNA consumption saving
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Embodiment 1
[0052] Identification of copy number of FRT site in Flp-In host cell line by fluorescent quantitative PCR
[0053] Genomic DNA preparation
[0054] The obtained host cell line Flp-In-K562 was constructed according to the operation steps of the Flp-InTMComplete System (Product No.: K601001) kit of Thermo Fisher Company. Genomic DNA of the host cell line Flp-In-K562 transformed with the pFRT / lacZeo plasmid was extracted. Genomic DNA was extracted with reference to the QIAGEN QIAamp DNA mini kit, and the DNA quality was detected by 1% agarose gel electrophoresis. 2 O was uniformly diluted to 50ng / μl. Genome electrophoresis results such as Figure 10 As shown, the extracted DNA bands are complete without tailing and smearing phenomenon, and the OD260 / 280 value of the measured sample is 1.9, which meets the experimental requirements in the range of 1.8-2.0.
[0055] The fluorescent quantitative PCR reaction system is shown in Table 2.
[0056] Table 2 Fluorescent quantitative ...
Embodiment 2
[0072] The repeatability detection of method in embodiment 1
[0073] Re-extract the sample DNA, measure the copy number of the sample again according to the method in Example 1, and observe whether the copy number calculation method twice is repeatable. The results are shown in Table 4.
[0074] Table 4 Secondary detection results of copy number of 7 Flp-In-K562 host cell line samples
[0075] Sample serial number LAC mean CT value UCR average CT value ΔCt copy number 5 22.968 21.056 1.912 1 6 22.702 20.903 1.799 1 23 23.522 21.635 1.887 1 30 22.936 21.322 1.614 1 58 23.153 21.184 1.969 1 63 22.131 21.594 0.537 1 76 20.014 21.195 -1.181 5
[0076] It can be drawn from Table 4 that the results of the seven samples are completely consistent. It shows that the method for measuring the copy number of the FRT site in the Flp-In-K562 host cell line provided by the present invention has stable results an...
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Abstract
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