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天然和候选疫苗变异肠产毒性耐热毒素的纯化和特性分析。

Purification and Characterization of Native and Vaccine Candidate Mutant Enterotoxigenic Heat-Stable Toxins.

机构信息

Centre for Applied Biotechnology, Uni Research Environment, 5006 Bergen, Norway.

Department of Biological Sciences, University of Bergen, 5006 Bergen, Norway.

出版信息

Toxins (Basel). 2018 Jul 3;10(7):274. doi: 10.3390/toxins10070274.

DOI:10.3390/toxins10070274
PMID:29970812
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6071264/
Abstract

Enterotoxigenic (ETEC), which secretes the heat-stable toxin (ST) is among the four most important enteropathogens that cause moderate-to-severe diarrhea in children in low- and middle-income countries. ST is an intestinal molecular antagonist causing diarrhea and hence an attractive vaccine target. A non-toxic and safe ST vaccine should include one or more detoxifying mutations, and rigorous characterization of such mutants requires structurally intact peptides. To this end, we established a system for purification of ST and ST mutants by fusing the sequence encoding the mature ST peptide to the disulfide isomerase DsbC. A Tobacco Etch Virus protease cleavage site facilitates the proteolytic release of free ST with no additional residues. The purified ST peptides have the expected molecular masses, the correct number of disulfide bridges, and have biological activities and antigenic properties comparable to ST isolated from ETEC. We also show that free DsbC can assist in refolding denatured and misfolded ST in vitro. Finally, we demonstrate that the purification system can be used to produce ST mutants with an intact neutralizing epitope, that two single mutations, L9S and A14T, reduce toxicity more than 100-fold, and that the L9S/A14T double mutant has no measurable residual toxicity.

摘要

肠产毒性大肠杆菌(ETEC)是导致中低收入国家儿童中中度至重度腹泻的四大最重要病原体之一,它能分泌热稳定毒素(ST)。ST 是一种肠道分子拮抗剂,可引起腹泻,因此是一种有吸引力的疫苗靶标。无毒且安全的 ST 疫苗应包含一个或多个解毒突变,而此类突变体的严格表征需要结构完整的肽。为此,我们通过将成熟 ST 肽的编码序列与二硫键异构酶 DsbC 融合,建立了一个用于纯化 ST 和 ST 突变体的系统。烟草蚀纹病毒蛋白酶切割位点可促进无额外残基的游离 ST 的蛋白水解释放。纯化的 ST 肽具有预期的分子量、正确数量的二硫键,并且具有与从 ETEC 分离的 ST 相当的生物活性和抗原特性。我们还表明,游离的 DsbC 可协助体外复性变性和错误折叠的 ST。最后,我们证明该纯化系统可用于生产具有完整中和表位的 ST 突变体,两个单突变 L9S 和 A14T 使毒性降低 100 多倍,并且 L9S/A14T 双突变体没有可测量的残留毒性。

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