A method for obtaining gene-edited sheep by RNA-mediated specific knockout of double genes and its dedicated sgRNA
A species-specific, sheep-based technology, applied in DNA/RNA fragments, recombinant DNA technology, animal cells, etc., can solve the problems of high cost and technical requirements for genome modification and transformation of large animals, difficulty in cultivating new varieties, and long breeding cycle , to avoid biosafety problems, shorten the experimental cycle, and reduce the cost of the experiment
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Embodiment 1
[0042] Embodiment 1, preparation sgRNA and Cas9mRNA
[0043] 1. Design the target sequence and sgRNA that recognizes the target sequence
[0044] 1. Design the target sequence of sheep MSTN gene and the sgRNA that recognizes the target sequence
[0045] The partial sequence of the sheep MSTN gene is shown in Sequence 1 of the Sequence Listing. The 1st to 3rd nucleotides from the 5' end are start codons, the 4989th to 4991st nucleotides are stop codons, and the 4611st to 4991st nucleotides are Nucleotides are exon 3. The protein encoded by the sheep MSTN gene is shown in sequence 2 of the sequence listing.
[0046] Six sgRNAs were designed for the target sequence of the sheep MSTN gene (the target sequence is on exon 3 of the sheep MSTN gene), see the italic parts in MSTN-TF1 to MSTN-TF6 in Table 1.
[0047] 2. Design the target sequence of sheep FGF5 gene and the sgRNA that recognizes the target sequence
[0048] The full-length sequence of the sheep FGF5 gene is shown in ...
Embodiment 2
[0080] Example 2, sgRNA / Cas9 mRNA mutation efficiency detection
[0081] 1. Obtaining fertilized sheep eggs
[0082] 1. Oocyte maturation
[0083] Collect sheep ovaries from the slaughterhouse (the ovaries are from Kazakh sheep), wash them with normal saline for 3-4 times, extract the oocytes, wash them with maturation solution for 3-4 times, and then drop them into well-balanced maturation solution (maturation solution The volume of the drop is 75-78μl, and each drop is filled with 25-30 oocytes), and placed in a solution containing 5% CO 2 cultured in a 38.6°C incubator (the following incubator cultures are all under the same conditions).
[0084] Equilibrate the mature solution: place the mature solution drop in the incubator for 2h. Maturation solution: TCM199 culture solution + 10% by volume FBS + 0.05IU / ml FSH + 0.05IU / ml LH + 1μg / ml estradiol + 24.2μg / ml sodium pyruvate + 0.1mM / L cysteine +10ng / ml EGF+100IU / ml penicillin+100IU / ml streptomycin.
[0085] 2. In vitro ...
Embodiment 3
[0111] Example 3, Production of gene-edited sheep
[0112] 1. Selection of experimental sheep
[0113] Xinjiang fine-wool sheep with good body condition, no reproductive diseases and 2-4 years old were selected as donor ewes. Select the Altay sheep with a weight of more than 50kg, an age of 2-4 years, good body condition and no reproductive diseases as recipient ewes. Select purebred Xinjiang fine-wool sheep with a body weight of 70-85kg, excellent semen detection and 1-3 years old as semen collection rams.
[0114] 2. Synchronous estrus and superovulation
[0115] During the estrous cycle of the sheep, the donor ewes were put into the vagina of the CIDR vaginal suppository, and on the 10th day after the CIDR vaginal suppository was put in, FSH (Ningbo Sansheng Company, China) was injected continuously in a decreasing manner, once every 12 hours, for a total of 3 days , the total dose is 240 units / only, take out the CIDR suppository in the morning of the 12th day, wash the ...
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