国际标准期刊号: 2155-952X

生物技术与生物材料

开放获取

我们集团组织了 3000 多个全球系列会议 每年在美国、欧洲和美国举办的活动亚洲得到 1000 多个科学协会的支持 并出版了 700+ 开放获取期刊包含超过50000名知名人士、知名科学家担任编委会成员。

开放获取期刊获得更多读者和引用
700 种期刊 15,000,000 名读者 每份期刊 获得 25,000 多名读者

索引于
  • 哥白尼索引
  • 谷歌学术
  • 夏尔巴·罗密欧
  • 打开 J 门
  • Genamics 期刊搜索
  • 学术钥匙
  • 研究圣经
  • 中国知网(CNKI)
  • 访问全球在线农业研究 (AGORA)
  • 电子期刊图书馆
  • 参考搜索
  • 哈姆达大学
  • 亚利桑那州EBSCO
  • OCLC-世界猫
  • SWB 在线目录
  • 虚拟生物学图书馆 (vifabio)
  • 普布隆斯
  • 日内瓦医学教育与研究基金会
  • 欧洲酒吧
  • ICMJE
分享此页面

抽象的

Cloning and Expression of Vaccine Peptide Containing NS3, E2, NS5A Genes of Hepatitis C Virus in Pichia Pastoris

Saeed Amel Jamehdar, Reza Karimi, Arezoo Esmaili, Samira Tabaei, Baratali Mashkani

Introduction: Hepatitis C is one of the most important causes of chronic hepatitis in developed countries. So far, no useful studies have been performed to design a cost-effective, high-immunity immunization vaccine for hepatitis C virus (HCV) infection. The aim of this study was to clone and express the vaccine peptide containing the NS3, E2, NS5A genes of hepatitis C virus in the yeast of Pichia pastoris.

Materials and methods: In this study, we used the methylotrophic yeast Pichia pastoris as our host to make the recombinant protein. In the next step, the dominant immuno-peptide genes NS3, NS5A and E2 were selected. The mouse IgG2a was selected as desired protein fraction. Linker peptide -GGGGS- was used to make the fusion peptide. The peptides were optimized using Geneious and Gen Script software before synthesis. Then, these genes were cloned into the expression vector pPICZαA. Pastoris strain GS115 strain was transferred to P. pastoris host cells.

Results: Spot blotting and SDS-PAGE techniques confirmed the expression of high levels of NS3-NS5A-E2 -Fc fusion peptide. The results of the other part of the study showed that the possibility of high protein expression is associated with the Codon Compatibility Index (CAI). The CAI of FC-NS3 -E2-NS5A components for Pichia pastoris expression host was 0.68. The other part of the study also showed that after optimizing the GC content became more uniform during the coding sequence. The results also showed that 39% of FC-NS3 -E2-NS5A codons were in the range of 91-100 codons (higher frequency codons) before optimization and this percentage reached 82% after gene optimization.

Conclusion: As a result, this study showed that fusion peptide is expressed in GS115 strains, as confirmed by dot blot technique.

免责声明: 此摘要通过人工智能工具翻译,尚未经过审核或验证。