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分析影响沙门氏菌血清型 Typhimurium 依赖 FlgM 的 III 型分泌系统进行蛋白质纯化的因素。

Analysis of factors that affect FlgM-dependent type III secretion for protein purification with Salmonella enterica serovar Typhimurium.

机构信息

Department of Biology, University of Utah, Salt Lake City, Utah, USA.

Department of Biology, University of Utah, Salt Lake City, Utah, USA

出版信息

J Bacteriol. 2014 Jul;196(13):2333-47. doi: 10.1128/JB.01572-14. Epub 2014 Apr 4.

Abstract

The FlgM protein is secreted in response to flagellar hook-basal body secretion and can be used as a secretion signal to direct selected protein secretion via the flagellar type III secretion (T3S) system [H. M. Singer, M. Erhardt, A. M. Steiner, M. M. Zhang, D. Yoshikami, G. Bulaj, B. M. Olivera, and K. T. Hughes, mBio 3(3):e00115-12, 2012, http://dx.doi.org/10.1128/mBio.00115-12]. Conditions known to affect flagellar gene expression, FlgM stability, and flagellar T3S were tested either alone or in combination to determine their effects on levels of secreted FlgM. These conditions included mutations that affect activity of the flagellar FlhD4C2 master regulatory protein complex or the FlgM T3S chaperone σ(28), the removal of Salmonella pathogenicity island 1 (Spi1), the removal of flagellar late secretion substrates that could compete with FlgM for secretion, and changes in the ionic strength of the growth medium. Conditions that enhanced FlgM secretion were combined in order to maximize levels of secreted FlgM. An optimized FlgM secretion strain was used to secrete and isolate otherwise difficult-to-produce proteins and peptides fused to the C terminus of FlgM. These include cysteine-rich, hydrophobic peptides (conotoxins δ-SVIE and MrVIA), nodule-specific, cysteine-rich antimicrobial peptides (NCR), and a malaria surface antigen domain of apical membrane antigen AMA-1.

摘要

FlgM 蛋白是在鞭毛钩-基体分泌的反应中被分泌出来的,可以作为一个分泌信号,通过鞭毛型 III 分泌(T3S)系统[H.M.Singer、M.Erhardt、A.M.Steiner、M.M.Zhang、D.Yoshikami、G.Bulaj、B.M.Olivera 和 K.T.Hughes,mBio 3(3):e00115-12,2012,http://dx.doi.org/10.1128/mBio.00115-12]来指导特定蛋白的分泌。已知会影响鞭毛基因表达、FlgM 稳定性和鞭毛 T3S 的条件被单独或组合进行测试,以确定它们对分泌的 FlgM 水平的影响。这些条件包括影响鞭毛 FlhD4C2 主调控蛋白复合物或 FlgM T3S 伴侣蛋白 σ(28)活性的突变、沙门氏菌致病岛 1(Spi1)的缺失、与 FlgM 竞争分泌的鞭毛晚期分泌底物的缺失,以及生长培养基离子强度的变化。增强 FlgM 分泌的条件被组合起来,以最大限度地提高分泌的 FlgM 水平。优化的 FlgM 分泌菌株被用于分泌和分离融合到 FlgM C 末端的其他难以生产的蛋白质和肽。这些包括富含半胱氨酸的疏水性肽(conotoxin δ-SVIE 和 MrVIA)、结节特异性、富含半胱氨酸的抗菌肽(NCR)和疟原虫表面抗原顶端膜抗原 AMA-1 的一个结构域。

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