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Presenting a foreign antigen on live attenuated Edwardsiella tarda using twin-arginine translocation signal peptide as a multivalent vaccine

机译:使用双精氨酸易位信号肽作为多价疫苗在减毒活的爱德华氏菌中呈递外源抗原

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The twin-arginine translocation (Tat) system is a major pathway for transmembrane translocation of fully folded proteins. In this study, a multivalent vaccine to present foreign antigens on live attenuated vaccine Edwardsiella tarda WED using screened Tat signal peptide was constructed. Because the Tat system increases the yields of folded antigens in periplasmic space or extracellular milieu, it is expected to contribute to the production of conformational epitope-derived specific antibodies. E. tarda Tat signal peptides fused with the green fluorescent protein (GFP) was constructed under the control of an in vivo inducible dps promoter. The resulting plasmids were electroporated into WED and the subcellular localizations of GFP were analyzed with Western blotting. Eight signal peptides with optimized GFP translocation efficiency were further fused to a protective antigen glyceraldehyde-3-phosphate dehydrogenase (GapA) from a fish pathogen Aeromonas hydrophila. Signal peptides of DmsA, NapA, and SufI displayed high efficiency for GapA translocation. The relative percent survival (RPS) of turbot was measured with a co-infection of E. tarda and A. hydrophila, and the strain with DmsA signal peptide showed the maximal protection. This study demonstrated a new platform to construct multivalent vaccines using optimized Tat signal peptide in E. tarda.
机译:双精氨酸易位(Tat)系统是全折叠蛋白跨膜易位的主要途径。在这项研究中,构建了一种多价疫苗,利用已筛选的Tat信号肽在减毒活的爱德华氏菌WED疫苗上呈递外源抗原。由于Tat系统提高了周质空间或细胞外环境中折叠抗原的产量,因此有望有助于构象表位衍生的特异性抗体的产生。在体内可诱导的dps启动子的控制下,构建了与绿色荧光蛋白(GFP)融合的E. tarda Tat信号肽。将所得质粒电穿孔到WED中,并用Western印迹分析GFP的亚细胞定位。将具有最佳GFP转运效率的八个信号肽进一步融合到鱼类病原体嗜水气单胞菌的保护性抗原甘油醛-3-磷酸脱氢酶(GapA)。 DmsA,NapA和SufI的信号肽显示出高效率的GapA易位。用塔氏大肠杆菌和嗜水链球菌的共同感染测定了菱turbo的相对存活百分率(RPS),并且带有DmsA信号肽的菌株显示出最大的保护作用。这项研究证明了一个新平台,可在塔氏大肠杆菌中使用优化的Tat信号肽构建多价疫苗。

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