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Co-expression with the Type 3 Secretion Chaperone CesT from Enterohemorrhagic E. coli Increases Accumulation of Recombinant Tir in Plant Chloroplasts

机译:与肠出血性大肠杆菌的3型分泌伴侣CesT的共表达增加植物叶绿体中重组Tir的积累。

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摘要

Type 3 secretion systems (T3SSs) are utilized by pathogenic Escherichia coli to infect their hosts and many proteins from these systems are affected by chaperones specific to T3SS-containing bacteria. Toward developing a recombinant vaccine against enterohaemorrhagic E. coli (EHEC), we expressed recombinant T3SS and related proteins from predominant EHEC serotypes in Nicotiana chloroplasts. Nicotiana benthamiana were transiently transformed to express chloroplast-targeted Tir, NleA, and EspD from the EHEC serotype O157:H7; a fusion of EspA proteins from serotypes O157:H7 and O26:H11; and a fusion of epitopes of Tir (Tir-ep) from serotypes O157:H7, O26:H11, O45:H2, and O111:H8. C-terminal GFP reporter fusion constructs were also developed and transiently expressed to confirm subcellular localization and quantify relative expression levels in situ. Recombinant proteins were co-expressed with chaperones specific to each T3SS protein with the goal of increasing their accumulation in the chloroplast. We found that co-expression with the chloroplast-targeted chaperone CesT significantly increases accumulation of recombinant Tir when the latter is either transiently expressed in the nucleus and targeted to the chloroplast of N. benthamiana or stably expressed in transplastomic Nicotiana tabacum. CesT also helped maintain higher levels of Tir:GFP fusion protein over time both in vivo and ex vivo, indicating that the favorable effect of CesT on accumulation of Tir is not specific to a single time point or to fresh material. By contrast, T3SS chaperones CesT, CesAB, CesD, and CesD2 did not increase accumulation of NleA:GFP, EspA:GFP, or EspD:GFP, which suggests dissimilar functioning of these chaperone–substrate combinations. CesT did not increase accumulation of Tir-ep:GFP, which may be due to the absence of the CesT binding domain from this fusion protein. The fusion to GFP improved accumulation of Tir-ep relative to the unfused protein, but not for the other recombinant proteins. These results emphasize the importance of native chaperones and stabilizing fusions as potential tools for the production of higher levels of recombinant proteins in plants; and may have implications for understanding interactions between T3SS chaperones and their substrates. In particular, our findings highlight the potential of T3SS chaperones to increase accumulation of recombinant T3SS proteins in heterologous systems.
机译:致病性大肠杆菌利用3型分泌系统(T3SS)感染其宿主,这些系统中的许多蛋白质均受特异于含T3SS细菌的分子伴侣的影响。为了开发针对肠出血性大肠杆菌(EHEC)的重组疫苗,我们从烟草叶绿体中表达了主要EHEC血清型的重组T3SS和相关蛋白。将本氏烟草瞬时转化为表达来自EHEC血清型O157:H7的叶绿体靶向的Tir,NleA和EspD;来自血清型O157:H7和O26:H11的EspA蛋白的融合体;以及来自血清型O157:H7,O26:H11,O45:H2和O111:H8的Tir(Tir-ep)表位的融合。还开发了C端GFP报告基因融合构建体,并瞬时表达以确认亚细胞定位并量化原位相对表达水平。重组蛋白与特异于每种T3SS蛋白的伴侣蛋白共表达,目的是增加它们在叶绿体中的积累。我们发现,当重组Tir在细胞核中瞬时表达并靶向本氏烟草的叶绿体或在转质体烟草中稳定表达时,与叶绿体靶向的伴侣CesT的共表达显着增加了重组Tir的积累。 CesT还可以在体内和离体的时间内帮助维持较高水平的Tir:GFP融合蛋白水平,这表明CesT对Tir积累的有利作用并非特定于单个时间点或新鲜材料。相比之下,T3SS伴侣CesT,CesAB,CesD和CesD2不会增加NleA:GFP,EspA:GFP或EspD:GFP的积累,这表明这些伴侣-底物组合的功能不同。 CesT不会增加Tir-ep:GFP的积累,这可能是由于该融合蛋白缺乏CesT结合域。相对于未融合的蛋白,与GFP的融合改善了Tir-ep的积累,但其他重组蛋白则没有。这些结果强调了天然伴侣蛋白和稳定融合蛋白作为在植物中生产更高水平的重组蛋白的潜在工具的重要性。可能对理解T3SS分子伴侣及其底物之间的相互作用有影响。特别地,我们的发现突出了T3SS分子伴侣增加异源系统中重组T3SS蛋白质积累的潜力。

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