A kind of reagent and its application for constructing free dna library
A DNA library and reagent technology, applied in the field of reagents for constructing cell-free DNA libraries, can solve problems such as interfering with embryo-derived DNA signals, and achieve the effects of shortening library construction time, shortening detection time, and reducing library construction costs.
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Embodiment 1
[0076] The present embodiment prepares mouse blastocyst culture liquid sample, comprises the following steps:
[0077] (1) Embryos are fertilized, and fertilized eggs are obtained according to the standard IVF cycle operation procedure of the reproductive center;
[0078] (2) Embryo transfer and single blastocyst culture, transfer the embryos to the marked blastocyst culture dish for single droplet culture (culture medium volume 20 μL);
[0079] (3) Collection of samples of blastocyst culture fluid. Place the embryos after the fluid change in the incubator to continue culturing. When the blastocysts develop to stage 4, evaluate the grade of the embryos, select embryos with 4CB / 4BC or above, and the blastocysts are fully expanded, and collect the corresponding ones. blastocyst culture medium;
[0080] Take 10 tubes of blastocyst culture fluid samples of mouse embryos above stage 4 and mix them to a total of 200 μL, vortex and mix 3 times for 3 seconds each time, and then distr...
Embodiment 2
[0082] This embodiment utilizes the mouse blastocyst culture fluid prepared in Example 1 to construct a library, and the construction method of the library comprises the following steps:
[0083] (1) Sample Lysis
[0084] 1) Centrifuge the 0.2mL PCR tube containing the blastocyst culture solution sample at 2000 rpm for 10 s, place it on ice, prepare the system according to Table 4, vortex for 5 s, mix the solution and centrifuge at 2000 rpm for 10 s, synchronously Set negative control, replace blastocyst culture medium with nuclease-free water; positive control, replace blastocyst culture medium with 8 mouse blastocyst cells;
[0085] Table 4
[0086]
[0087] 2) Set the reaction program of the PCR instrument, and perform lysis as shown in Table 5.
[0088] table 5
[0089]
[0090] (2) End repair plus dA tail
[0091] 1) Add 19 μL of nuclease-free water and 1 μL of carrier DNA (SEQ ID NO.1) to the lysate of step (1);
[0092] 2) Prepare the end repair reaction soluti...
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