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鉴定鱼类迟缓爱德华氏菌弱毒血清型的亚单位疫苗抗原。

Identification of antigens for the development of a subunit vaccine against Photobacterium damselae ssp. piscicida.

机构信息

Institute of Biotechnology, National Cheng Kung University, Tainan 701, Taiwan.

出版信息

Fish Shellfish Immunol. 2011 Jan;30(1):412-9. doi: 10.1016/j.fsi.2010.11.029. Epub 2010 Dec 4.

Abstract

Photobacterium damselae ssp. piscicida (Ph.d.p.), the causative agent of photobacteriosis, is among the most important pathogens affecting finfish aquaculture globally. With the emergence of recombinant technology, subunit vaccines have been actively pursued, but mostly for viral diseases. Bacterial subunit vaccines are more difficult to develop since the bacterial genome is more complex, with numerous candidate antigens, leading to a lengthy and laborious screening process. Immunoproteomics, using western blotting on protein analyzed with 2DE and LC-MS/MS to isolate immune-reactive proteins and acquire amino acid sequences, followed by recombinant technology to clone the candidate gene, identified eight candidate antigens from Ph.d.p., which have been cloned and expressed in Escherichia coli BL21(DE3). These proteins were purified and used as antigens in an efficacy trial. Three, rHSP60, rENOLASE, and rGAPDH proteins, elicited higher specific antibody titers and stronger protective immunity than the other five and an inactivated Ph.d.p. whole bacterial vaccine. These three antigens may be candidates for the development of a subunit vaccine against Ph.d.p.

摘要

美人鱼发光杆菌亚种(Ph.d.p.)是一种引起发光病的病原体,是目前全球影响鱼类养殖最重要的病原体之一。随着重组技术的出现,亚单位疫苗的研究已经得到了积极的推进,但主要还是针对病毒性疾病。由于细菌基因组更加复杂,存在众多候选抗原,因此细菌亚单位疫苗的开发更加困难,这导致筛选过程漫长而繁琐。免疫蛋白质组学使用 2DE 和 LC-MS/MS 分析的蛋白质进行 Western blot,以分离免疫反应性蛋白并获取氨基酸序列,然后通过重组技术克隆候选基因,从 Ph.d.p. 中鉴定出 8 种候选抗原,这些抗原已在大肠杆菌 BL21(DE3)中克隆和表达。这些蛋白被纯化并用作功效试验中的抗原。三种蛋白,rHSP60、rENOLASE 和 rGAPDH,比其他五种蛋白和一种灭活的 Ph.d.p.全细菌疫苗诱导出更高的特异性抗体滴度和更强的保护免疫。这三种抗原可能是开发针对 Ph.d.p.的亚单位疫苗的候选抗原。

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