A[beta]42-modified protein with function of resisting protein aggregation and expression and purification methods thereof
A protein aggregation and protein technology, applied in the fields of biotechnology and genetic engineering, can solve problems such as aggregation characteristics and toxicity research
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Embodiment 1
[0077] Example 1: pET22b-His 6 -Aβ42 expression vector plasmid and recombinant His 6 - Construction of Aβ42 Escherichia coli expression strain
[0078] His 6 - Aβ42 expression and purification flow chart as shown figure 1 shown;
[0079] Expression vector pET22b-His 6 -Aβ42 construction schematic diagram as shown in figure 2 shown;
[0080] (1) Perform codon optimization on the Aβ42 gene sequence according to the amino acid sequence of Aβ42 and the codon preference of Escherichia coli to obtain the amino acid sequence of Aβ42 such as SEQ ID No.3 and the nucleotide sequence such as SEQ ID No.4;
[0081] (2) Using primer NdeⅠ-His 6 -Aβ42-F and XhoⅠ-His 6 -Aβ42-R, the primer sequences are shown in SEQ ID No.5 and SEQ ID No.6. The upstream primer NdeⅠ-His 6 -Aβ42-F contains His 6 The gene sequence of the tag, add His at the upstream of the Aβ42 gene sequence by PCR 6 tag, get His 6 -Aβ42 target gene sequence as shown in SEQ ID No.2, His 6 - The amino acid sequence o...
Embodiment 2
[0096] Example 2: His 6 -Expression and purification of Aβ42 protein
[0097] His 6- Aβ42 expression and purification flow chart as shown figure 1 shown.
[0098] (1)His 6 -Aβ42 protein expression: use 1mM isopropyl-β-D-thiogalactopyranoside to induce protein expression, and the engineering bacteria BL21-His obtained in Example 1 6 -Aβ42 was induced at 30°C for 20 hours. After the induction, the bacterial liquid was centrifuged to collect the bacterial cells to obtain 6 -Escherichia coli thalline of Aβ42 fusion protein;
[0099] (2) His 6 -Purification of Aβ42 protein: Resuspend the bacteria obtained above with buffer, add 1% phenylmethylsulfonyl fluoride, sonicate after 30 minutes in ice bath, and centrifuge at 12000 rpm for 30 minutes. 6 -Aβ42 protein is mainly expressed in the form of inclusion bodies, and the inclusion bodies are denatured and dissolved by using buffer A solution containing urea.
[0100] The composition of the denaturing solution (buffer A) is: 20...
Embodiment 3
[0106] Example 3: His 6 -Aβ42 peptide identification
[0107] (1) Electrophoretic identification: the His prepared in Example 2 of the present invention 6 - The purity and molecular weight of Aβ42 protein were determined by SDS-PAGE electrophoresis, such as image 3 As shown, there is an obvious band around 5.47kDa. The protein concentration was detected by the NanoDrop 2000 protein and nucleic acid quantitator, and the final calculation of 1L bacterial solution can obtain about 22mg His 6 - Aβ42 polypeptide.
[0108] (2) Mass spectrometry identification: the purified His 6 -Aβ42 polypeptide was identified by MALDI TOF mass spectrometry, such as Figure 4 As shown, the peak with a charge-to-mass ratio of 5470 is His 6 -Aβ42 polypeptide, so it can be proved that this protein is the target protein His 6 - Aβ42.
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