Mutant Alfimeprase engineering strain, and preparation method and applications thereof
A technology of engineering strains and plasmin, applied in the biological field, can solve problems such as oxidation, re-embolization, and limited sources of raw materials, and achieve high activity and stable strains
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Embodiment 1
[0028] Using the amino acid sequence (GenBank No.P28891) of the venom Fibrolase protein published by the National Center for Biotechnology (NCBI) in the United States, the EQR at its N-terminal was mutated into serine S, and its amino acid sequence was shown in SEQ ID No. .1 shown. Combined with the codon bias of eukaryotic organisms, the nucleotide sequence is designed, and the nucleotide sequence is shown in SEQ ID No.2.
[0029] Four rounds of PCR reactions were used to obtain the gene fragment encoding Alfimeprase containing the required restriction enzyme site, His×6 tag, and EK site. The PCR schematic diagram is as follows figure 1 shown. The reaction system used in each round of PCR is as follows:
[0030] The first round of PCR with SEQ ID No.3 and SEQ ID No.4, SEQ ID No.5 and SEQ ID No.6, SEQ ID No.7 and SEQ ID No.8, SEQ ID No.9 and SEQ ID No. .10, SEQ ID No.11 and SEQ ID No.12, SEQ ID No.13 and SEQ ID No.14, SEQ ID No.15 and SEQ ID No.16 are primers for PCR amplif...
Embodiment 2
[0091] according to Figure 4 The method shown was used to construct the expression vector pPic9K-His-Alf. The pBS-Alf constructed in Example 1 and the expression vector pPIC9K were digested with EcoR I and Not I ( Figure 5 ), purify and collect the digested fragments, and connect them to obtain the recombinant expression vector pPIC9K-His6-Alf. The double digestion and connection system are as follows:
[0092] Enzyme digestion reaction system 1: Enzyme digestion reaction system 2:
[0093] pBS-Alf plasmid 10μl pPIC9k plasmid 10μl
[0094] EcoR I (12u / μl) 2.0μl EcoR I (12u / μl) 1.5μl
[0095] Not I (10u / μl) 2.0μl Not I (10u / μl) 1.5μl
[0096] 10x Digestion Buffer 6μl 10x Digestion Buffer 6μl
[0097] 10xBSA 6μl 10xBSA 6μl
[0098] Sterile water 34μl Sterile water 34.5μl
[0099] Total volume 60μl Total volume 60μl
[0100] Connection reaction system:
[0101] Recover 1.5 μl of purified pPIC9K plasmid
[0102] Recover and purify the target fragment His6-Alf 5 μl
[...
Embodiment 3
[0108] Shake flask culture in BMG / MY liquid medium, liquid volume 100ml, shaker speed 250rpm, when the OD600 value reaches 1-1.5, add sterile methanol 1-2ml to induce expression, then add once every 24 hours . Sampling was carried out continuously for electrophoresis determination, and cultured for 5 days.
[0109] Collect the fermentation broth, centrifuge at 10,000 rpm, concentrate in vacuum at low temperature, gradually add ammonium sulfate to the concentrated solution to a final concentration of 50%, and keep stirring gently, centrifuge the precipitate at 3,000 rpm, remove the supernatant, and redissolve the precipitate with physiological saline. The solution was purified according to the operating instructions of the His-Bind protein purification kit from Novagen. The purified protein solution was collected, cut with enterokinase EK, precipitated with ammonium sulfate again, centrifuged, precipitated and dialyzed for redissolution to obtain active Alfimeprase.
[0110] ...
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