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利用基于连接独立克隆的、SOS 诱导表达系统鉴定新型炭疽杆菌种间血清反应性蛋白。

Identification of novel and cross-species seroreactive proteins from Bacillus anthracis using a ligation-independent cloning-based, SOS-inducible expression system.

机构信息

Alkek Center for Metagenomics and Microbiome Research, Department of Molecular Virology and Microbiology, Baylor College of Medicine, One Baylor Plaza, Houston, TX 77030, USA.

出版信息

Microb Pathog. 2012 Nov-Dec;53(5-6):250-8. doi: 10.1016/j.micpath.2012.08.006. Epub 2012 Sep 10.

Abstract

The current standard for Bacillus anthracis vaccination is the Anthrax Vaccine Adsorbed (AVA, BioThrax). While effective, the licensed vaccine schedule requires five intramuscular injections in the priming series and yearly boosters to sustain protection. One potential approach to maintain or improve the protection afforded by an anthrax vaccine, but requiring fewer doses, is through the use of purified proteins to enhance an antibody response, which could be used on their own or in combination with the current vaccine. This study describes a novel, high-throughput system to amplify and clone every gene in the B. anthracis pXO1 and pXO2 virulence plasmids. We attempted to express each cloned gene in Escherichia coli, and obtained full-length expression of 57% of the proteins. Expressed proteins were then used to identify immunogens using serum from three different mammalian infection models: Dutch-belted rabbits, BALB/c mice, and rhesus macaque monkeys. Ten proteins were detected by antibodies in all of these models, eight of which have not been identified as immunoreactive in other studies to date. Serum was also collected from humans who had received the AVA vaccine, and similar screens showed that antigens that were detected in the infection models were not present in the serum of vaccinated humans, suggesting that antibodies elicited by the current AVA vaccine do not react with the immunoreactive proteins identified in this study. These results will contribute to the future selection of targets in antigenicity and protection studies as one or more of these proteins may prove to be worthy of inclusion in future vaccine preparations.

摘要

炭疽杆菌疫苗接种的现行标准是吸附型炭疽疫苗(AVA,BioThrax)。虽然该疫苗有效,但许可的疫苗接种方案需要在初级系列中进行五次肌肉内注射,并每年加强针以维持保护。一种保持或提高炭疽疫苗保护效果但需要更少剂量的潜在方法是使用纯化蛋白来增强抗体反应,这些蛋白可以单独使用或与当前疫苗联合使用。本研究描述了一种新颖的高通量系统,可扩增和克隆炭疽杆菌 pXO1 和 pXO2 毒力质粒中的每个基因。我们试图在大肠杆菌中表达每个克隆的基因,并获得了 57%的蛋白质全长表达。然后使用这些表达的蛋白质来鉴定来自三种不同哺乳动物感染模型的血清中的免疫原:荷兰兔、BALB/c 小鼠和恒河猴。在所有这些模型中,有 10 种蛋白质被抗体检测到,其中 8 种在迄今为止的其他研究中未被鉴定为具有免疫反应性。还从接种了 AVA 疫苗的人类中收集了血清,类似的筛选表明,在感染模型中检测到的抗原不存在于接种疫苗的人类血清中,这表明当前 AVA 疫苗引发的抗体不会与本研究中鉴定的免疫反应性蛋白发生反应。这些结果将有助于未来在抗原性和保护研究中选择目标,因为其中一种或多种蛋白质可能被证明值得包含在未来的疫苗制备中。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2472/3779308/f981871531cc/nihms471547f1.jpg

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