Bacteria one-hybrid vector and preparation
A carrier and bacterial technology, applied in the field of bacterial single-hybrid reporter carrier, to inhibit self-activation and facilitate rapid cloning
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Embodiment 1
[0030] The preparation of embodiment 1 carrier of the present invention
[0031] 1. Obtain the reporter gene His3-aadA fragment
[0032] The total DNA of the bacterial two-hybrid system reporter strain XL1-Blue MRF'Kan (purchased from Stratagene) was used as the template, and Rpb-f (5'-TAGAGGATCCTTGTCGAAGATCTTCGACAAC-3' and Rpb-r (5'-GAACCTCGAGTTATTTGCCAACTACCTTAGTGATCTCG-3') were used as templates. Primers carried out PCR amplification PCR amplification, obtained the His3-aadA reporter gene fragment of about 1.7kb, the obtained PCR product was cloned into pBS-T vector (purchased from TIANGEN company), positive clone corresponding sample sequencing (by INVITROGEN sequencing ) to verify the correctness of the target PCR product.
[0033] The PCR process is as follows:
[0034] Reaction system: Reaction procedure:
[0035] 2×GC Buffer I 37.5μl 96℃ 5min;
[0036] 2.5mM dNTP 8μl 94℃ 50sec;
[0037] Rpb-f 2μl 57℃ 50sec;
[0038] Rpb-r 2μl 72℃ 2min;
[0039] Genomic DNA 2μl 3...
Embodiment 2
[0076] Embodiment 2: Carry out the method for high-throughput bacterial one-hybrid screening with pBXcmT carrier (biological application embodiment)
[0077] 1. Preparation of screening medium:
[0078] The reagents used in the screening medium of the present invention were all purchased from Stratagene Company.
[0079] (1) Accurately weigh 7.5g of agar powder, adjust the volume to 380mL with distilled water, adjust the pH to 6.8-7.0, sterilize at 121°C for 20 minutes, and keep it warm for later use;
[0080] (2) When the agar is cooled to 70°C, quickly add 50mL of 10×M9 salts and mix well;
[0081] (3) When the above mixture is cooled to 50°C, quickly add 67.5mL M9media additive, 0.5mL chloramphenicol (34mg / mL), 0.5mL tetracycline (12.5mg / mL), 10mL 3-AT (1M), 1mL streptavidin Vegetable (8mg / mL), mix quickly;
[0082] (4) Quickly pour the uniformly mixed culture medium onto a plate to form a screening plate, and place the plate at 4°C for standby (storage time shall not ex...
Embodiment 3
[0087] Example 3: Functional verification of the initial carrier pRpb
[0088]According to the documents already published by the applicant (Jiang PX, Feng Y, He ZG Functional differentiation and cooperative interaction between two eukaryote-like archaeal Orc1 / Cdc6 proteins on thereplication origin. Biochem Biophys Res Commun. 2007Dec 28; 364 (4): 945- 51), the specific interaction between the replication initiation protein Cdc6 of the extreme thermophilic archaea Sulfolobus solfataricus P2 and the replication origin Ori1, and the C-terminus of Cdc62 is responsible for this interaction. However, in vitro experiments showed that the protein (Cdc 62Δc) after deletion of the C-terminus of Cdc62 still retained part of the function of interacting with Ori1. Therefore, the present invention selects S. solfataricus P2 replication initiation protein Cdc61, Cdc62, Cdc62Δc (C-terminal deletion of Cdc62) gene and S. solfataricus P2 replication origin Ori1 sequence respectively cloned int...
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