A kind of meningitis polysaccharide conjugate vaccine with heterotype bifunctional reagent as connecting bridge and preparation method thereof
一种结合疫苗、荚膜多糖的技术,应用在生物医药领域,能够解决降低多糖-蛋白结合效率、多糖与载体蛋白自身交联、限制多糖结合疫苗发展等问题,达到提高免疫原性、减小空间屏蔽效应、利于质量控制的效果
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Embodiment 1
[0035] Example 1: Preparation of polysaccharide conjugate vaccine
[0036] Preparation of polysaccharide conjugate vaccine without PEG (PS-TT), polysaccharide conjugate vaccine with PEG2K as bridge (PS-P2K-TT), and polysaccharide conjugate vaccine with PEG5K as bridge (PS-P5K-TT) react as figure 1 shown. Dissolve 10 mg of group Y meningococcal capsular polysaccharide in 2 ml of normal saline, add 20 μL of cyanogen bromide solution (w / v 50%) for activation, and react at room temperature for 1 hour. During activation, the pH of the solution was maintained at 10.5 with 0.5M NaOH. After the activation, the pH value of the solution was adjusted to 8.5 with 0.5M hydrochloric acid to terminate the reaction. Subsequently, 10 mg N-2-aminoethyl-maleimide, 60 mg amine-PEG2K-maleimide (PEG molecular weight 2 kDa) and 75 mg amine-PEG5K-maleimide (PEG molecular weight 5 kDa) were added separately ). React overnight at room temperature. After the reaction, use a filter membrane with a ...
Embodiment 2
[0038] Example 2: Characterization of three polysaccharide conjugate vaccines
[0039] The polysaccharide-protein combination product involved in Example 1 was separated and purified with a Superdex200 gel filtration column (2.6cm×60cm), the eluent was 20mM phosphate buffer (pH7.4), and the flow rate was 3ml / min . Elution peaks corresponding to PS-TT, PS-P2K-TT and PS-P5K-TT were collected separately.
[0040] The purified product was identified by Superdex200 gel filtration column (1.0cm×30cm), the eluent was 20mM phosphate buffer (pH7.4), and the flow rate was 0.5ml / min. Such as figure 2 As shown, compared with the carrier protein, the peak time of PS-TT, PS-P2K-TT and PS-P5K-TT was significantly earlier. This indicates that the molecular weight of the carrier protein increases significantly after binding to the pneumonia capsular polysaccharide. Since the three combined products all elute in the outer water volume of the gel filtration column, the peak eluting times of...
Embodiment 3
[0042] Example 3: Determination of the immunogenicity of polysaccharide-conjugated vaccines
[0043] Select 32 5-week-old female Blab / C mice weighing 15-22 g. They were randomly divided into 4 groups, namely capsular polysaccharide group, PS-TT group, PS-P2K-TT group and PS-P5K-TT group, with 8 mice in each group. Intraperitoneal injection, each injection containing 5 micrograms of polysaccharides, once a week, a total of 3 injections. After 21 days, blood was collected from the orbit. Anti-capsular polysaccharide IgG, IgG1 and IgG2a in mouse plasma were detected by ELISA.
[0044] Such as Figure 4 As shown, the capsular polysaccharide group produced weak IgG and IgG1 titers against the capsular polysaccharide, while IgG2a was not detected. The antibody titer increased significantly after the capsular polysaccharide was coupled with the carrier protein. Compared with the capsular polysaccharide group, the anti-capsular polysaccharide IgG and IgG1 antibody titers in the P...
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