牛分枝杆菌BCG作为白喉毒素dtb基因抗原的递送系统

D. Nascimento, O. Dellagostin, D. S. Matos, D. McIntosh, R. Hirata, G. M. Pereira, A. Mattos-Guaraldi, G. R. Armôa
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摘要

白喉是一种由白喉棒状杆菌产毒菌株引起的暴发性细菌性疾病,其局部和全身表现是由于白喉毒素(DT)的作用。世界范围内用于预防白喉的疫苗是通过对DT进行解毒而获得的类毒素。尽管目前的抗白喉疫苗是DTP(白喉、破伤风和百日咳三联疫苗)的组成部分之一,在预防疾病方面具有很高的效力,但它可能会在接种后产生毒性和反应原性等影响,这些影响是由于疫苗中存在生产和/或解毒过程中产生的污染物所致。因此,需要制定一种毒性较小、同时在经济上可行的疫苗替代品的战略,以改进世界各地使用的现有疫苗。在本研究中,对巴西用作人类结核病活疫苗的BCG的Moreau亚基进行了基因修饰,以携带和表达白喉毒素片段B(DTB)的编码基因。因此,将编码dtb基因的DNA序列克隆到pUS977穿梭载体中用于细胞质表达,并通过电穿孔成功地引入BCG细胞中。用表达DTB的重组BCG免疫的小鼠在检测到针对DTB的特异性抗体时显示出血清转化。此外,在小鼠中没有选择性压力的情况下,稳定表达DTB的rBCG持续长达60天,并且在测试期间细胞活力没有显著变化。最后,在Vero细胞测定中,初步测试了接种rBCGpUS977dtbPW8的BALB/c小鼠的免疫血清中和白喉毒素的能力。
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Mycobacterium bovis BCG as a Delivery System for the dtb Gene Antigen from Diphtheria Toxin
Diphtheria is a fulminant bacterial disease caused by toxigenic strains of Corynebacterium diphtheriae whose local and systemic manifestations are due to the action of the diphtheria toxin (DT). The vaccine which is used to prevent diphtheria worldwide is a toxoid obtained by detoxifying DT. Although associated with high efficacy in the prevention of disease, the current anti-diphtheria vaccine, one of the components of DTP (diphtheria, tetanus and pertussis triple vaccine), may present post vaccination effects such as toxicity and reactogenicity resulting from the presence of contaminants in the vaccine that originated during the process of production and/or detoxification. Therefore, strategies to develop a less toxic and at the same time economically viable vaccine alternatives are needed to improve existing vaccines in use worldwide. In this study, the Moreau substrain of BCG which is used in Brazil as a live vaccine against human tuberculosis was genetically modified to carry and express the gene encoding for the diphtheria toxin fragment B (DTB). As such, the DNA sequence encoding the dtb gene was cloned into the pUS977 shuttle vector for cytoplasmic expression and successfully introduced into BCG cells by electroporation. Mice immunized with recombinant BCG expressing DTB showed seroconversion with the detection of specific antibodies against DTB. Also, rBCGs stably expressing DTB persisted up to 60 days in the absence of selective pressure in mice and cell viability did not change significantly during the period tested. Finally, immune sera from BALB/c mice vaccinated with rBCGpUS977dtbPW8 were preliminarily tested for their capacity of neutralizing the diphtheria toxin in the Vero Cells assay.
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