Purification method of candidate antigen glu of Streptococcus mutans recombinant subunit gene engineering vaccine
A technology of genetically engineered vaccine, Streptococcus mutans, which is applied in the field of purification of recombinant Streptococcus mutans dental caries vaccine candidate antigen Glu, which can solve the problems of body injury and insufficient attenuation
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Embodiment 1
[0041] Example 1 Preparation of Antigen Glu
[0042] (1) Cloning of Streptococcus mutans Glu gene
[0043] 1. Streptococcus mutans UA159 (from the American Type Culture Collection Center, ATCC) (preserved by the Department of Clinical Microbiology and Immunology, Third Military Medical University of the Chinese People's Liberation Army)
[0044] 2. Take out the preserved Streptococcus mutans UA159 strain from the liquid nitrogen tank, spread it on the BHI solid medium, and cultivate it overnight at 37°C. Genome extraction kit to extract the genome of Streptococcus mutans.
[0045] 3. Using the PCR method to amplify the Glu coding gene from the Streptococcus mutans genome respectively.
[0046] 1) The primers were designed and synthesized as follows (the base sequence of the restriction site is underlined)
[0047] According to the gene sequence published by GenBank and the principles of primer design, the corresponding primers were designed and restriction sites were intr...
Embodiment 2
[0145] Example 2 Autoclave, centrifuge
[0146] 1. Ferment the constructed Escherichia coli engineering bacteria expressing the Streptococcus mutans recombinant subunit genetically engineered protein Glu, and the expression rate of the target protein is 26%, and the bacteria are collected by centrifugation for later use.
[0147] 2. Mix and suspend 200-500 g of bacteria in PBS (10-20 mM, pH 7.0-7.5) buffer according to the weight: volume ratio of 1:10, and pre-cool at 4°C.
[0148] 3. High-pressure homogenizer: Use distilled water to flush the pipeline of the high-pressure homogenizer, and turn on the low-temperature circulation system to pre-cool to 1-4°C for standby.
[0149] 4. Add the pre-cooled suspended bacteria into a high-pressure homogenizer, maintain the pressure at 60-80Mpa to break the bacteria 3-5 times, take a smear of the broken bacteria and stain it with crystal violet, and the number of unbroken bacteria in each field of view under the oil microscope is less...
Embodiment 3
[0152] Example 3 Inclusion body washing and lysis
[0153] 1. Resuspend the centrifugal pellet with 9 times the volume of pH 7.0-7.520mM PB buffer containing 1% Triton X-100, and mix thoroughly with a high-speed disperser, then gently stir with a stirrer for 30min, and then Centrifuge at 10,000×g for 30 minutes, collect the precipitate, and repeat once;
[0154] 2. Resuspend the centrifuged pellet with 9 times the volume of pH 7.0-7.520mM PB buffer containing 2M urea, mix well with a high-speed disperser, stir gently with a stirrer for 15min, and then centrifuge at 10000×g for 30min. Collect the precipitate and repeat once;
[0155] 3. Weigh the wet weight of the precipitate, add PB (10-20mM, pH7.0-7.5) buffer solution containing 8M urea according to the weight: volume ratio of 1:10, stir and dissolve overnight at 4°C, centrifuge at 13000g for 30 minutes at high speed, and collect supernatant.
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