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Enhanced Murine Antigen-Specific Gamma Interferon and Immunoglobulin G2a Responses by Using Mycobacterial ESAT-6 Sequences in DNA Vaccines

机译:通过使用DNA疫苗中的分枝杆菌ESAT-6序列增强小鼠抗原特异性γ干扰素和免疫球蛋白G2a反应。

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摘要

The Mycobacterium tuberculosis protein ESAT-6 has unusual immune stimulating activities, has been implicated in the recall of long-lived immunity, and induces protection against tuberculosis in mice. For many diseases caused by bacterial or viral pathogens, a strong cell-mediated immune (i.e., type 1) response is often required for recovery or protection. Therefore, it is important to design immunization regimens that induce agent-specific type 1 immunity. We have shown in previous studies that ESAT-6 could enhance antigen-specific type 1 immune responses in BALB/c mice against a second antigen when presented as a purified fusion protein. It was also of interest to determine if ESAT-6 could enhance the type 1 response against a second antigen beyond that afforded by DNA vaccination through CpG motifs. This was tested by using gene fusions of ESAT-6 and the Mycoplasma hyopneumoniae surface antigen P71. Modified P71 gene sequences were cloned with or without ESAT-6 sequences into a DNA vaccine vector and were used to immunize mice. Splenic lymphocytes from vaccinated mice were tested for gamma interferon (IFN-γ) and interleukin-10 (IL-10) secretion. Serum antibodies were examined for P71 antigen-specific isotype responses. When stimulated in vitro with purified P71 antigen, splenocytes from the ESAT-6:P71 vaccinates secreted higher levels of IFN-γ and lower levels of IL-10 compared to those of vaccinates receiving the P71 construct alone. Furthermore, the immunoglobulin G2a serum antibody levels were significantly higher in the ESAT-6:P71 vaccinates compared to those of the vaccinates receiving P71 alone. In conclusion, ESAT-6 was shown to enhance antigen-specific type 1 immune responses in BALB/c mice when used in DNA vaccines.
机译:结核分枝杆菌蛋白ESAT-6具有异常的免疫刺激活性,与长期免疫的恢复有关,并能诱导小鼠抗结核病。对于由细菌或病毒病原体引起的许多疾病,恢复或保护通常需要强烈的细胞介导的免疫反应(即1型)。因此,设计诱导试剂特异的1型免疫的免疫方案很重要。在先前的研究中我们已经表明,当以纯化的融合蛋白形式存在时,ESAT-6可以增强BALB / c小鼠中针对第二种抗原的抗原特异性1型免疫应答。确定ESAT-6是否可以增强对第二种抗原的1型应答,这超出了通过CpG基序进行DNA疫苗接种所提供的应答。这是通过使用ESAT-6和猪肺炎支原体表面抗原P71的基因融合来测试的。将修饰的P71基因序列与有或没有ESAT-6序列一起克隆到DNA疫苗载体中,并用于免疫小鼠。测试了来自接种疫苗的小鼠的脾淋巴细胞的γ干扰素(IFN-γ)和白介素10(IL-10)的分泌。检查血清抗体的P71抗原特异性同种型反应。当用纯化的P71抗原体外刺激时,与单独接受P71构建体的疫苗相比,来自ESAT-6:P71疫苗的脾细胞分泌更高水平的IFN-γ和更低水平的IL-10。此外,与单独接受P71的疫苗相比,ESAT-6:P71疫苗中的免疫球蛋白G2a血清抗体水平明显更高。总之,当在DNA疫苗中使用ESAT-6时,可增强BALB / c小鼠的抗原特异性1型免疫应答。

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