Basic group editing tool and application thereof, and basic group editing method with wide window and no sequence preference in eukaryocyte
A technology of base editing and tools, applied in the field of base editing, which can solve the problems of limited application and achieve the effect of wide editing window and no sequence preference in the editing window
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[0040] According to the present invention, the sequence of the linker may be any amino acid sequence capable of connecting the amino acid sequences at both ends, and the present invention has no particular limitation on this. According to a preferred embodiment of the present invention, the linker The amino acid sequence of is shown in SEQ ID NO:1.
[0041]According to the present invention, the cytosine deaminase AID can be any amino acid sequence having cytosine deaminase AID activity known in the art, and according to a preferred embodiment of the present invention, the cytosine deaminase is The amino acid sequence of the full-length AIDfl is shown in SEQ ID NO:4.
[0042] However, the inventors of the present invention found in research that by performing point mutation and C-terminal truncation on the amino acid sequence shown in SEQ ID NO: 4, the base editing efficiency of the final base editing tool can be effectively improved, Wherein, the point mutation is selected f...
Embodiment 1
[0066] This example is used to illustrate the construction of a plasmid encoding scFv-AID-UGI-GB1 protein
[0067] 1. Amplification of nucleic acid sequence fragment (AID) encoding AID
[0068] The coding sequence hAID*Δ of the optimized version of cytosine deaminase AID hAID*Δ synthesized by Jinweizhi Biotechnology Co., Ltd. (the encoded amino acid sequence is shown in SEQ ID NO: 5, and the DNA sequence is shown in SEQ ID NO: 139) , cloned in the pUC57 vector to obtain the pUC57-hAID*Δ vector, diluted to 10 μM as a PCR template. Design forward primer (as shown in SEQ ID NO: 10), reverse primer (as shown in SEQ ID NO: 11), add water and dissolve to 10 μM. The hAID sequence fragment was amplified using Novizan High Fidelity Enzyme Kit (Vazyme, p501-d2). The amplification system is shown in Table 1, and the PCR reaction conditions are shown in Table 2.
[0069] Table 1
[0070]
[0071] Table 2
[0072]
[0073] 2. Amplification of the nucleic acid sequence fragment (...
Embodiment 2
[0087] This example is used to illustrate the construction of the plasmid encoding scFv-AIDfl-UGI-GB1 protein
[0088] The construction of the plasmid encoding the scFv-AIDfl-UGI-GB1 protein was carried out according to Example 1, except that the human codon-optimized hAID*Δ was replaced with the nucleotide sequence of the unoptimized full-length AIDfl, that is, the encoding For the nucleotide sequence (SEQ ID NO: 138) of the protein shown in SEQ ID NO: 4, the amplification forward primer and reverse primer are shown in SEQ ID NO: 143 and SEQ ID NO: 144, respectively, to obtain BE-PA2.
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