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Bacteriocinogenic Clo DF13 Minicells of Escherichia coli Synthesize a Protein That Accounts for Immunity to Bacteriocin Clo DF13: Purification and Characterization of the Immunity Protein

机译:大肠杆菌的致细菌致病性Clo DF13小细胞合成一种对致细菌性细菌Clo DF13具有免疫力的蛋白:免疫蛋白的纯化和鉴定

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摘要

Cloacin DF13 inhibits protein synthesis both in vivo and in vitro by inactivation of ribosomes. In this paper we describe the purification, from purified bacteriocinogenic plasmid DF13 (Clo DF13)-harboring minicells of Escherichia coli, of an acidic protein (molecular weight about 10,000) that prevents the inhibition of in vitro protein synthesis by cloacin DF13. It turned out that this protein is one of three Clo DF13 plasmid-specific polypeptides that are synthesized by the noninduced Clo DF13 plasmid in minicells. Furthermore, we observed that, after induction with mitomycin C, the amount of immunity protein is only slightly increased, whereas the cloacin DF13 synthesis is increased about 40 times. These results imply that the genes that code for immunity protein and cloacin DF13 are not located in the same regulatory unit. Under noninduced conditions, apparently an excess of immunity protein is synthesized, because this amount of immunity protein is even sufficient to neutralize the strongly increased amount of cloacin after induction, since growth of induced cloacinogenic cells is continued.
机译:Cloacin DF13通过使核糖体失活来抑制体内和体外的蛋白质合成。在本文中,我们描述了从纯化的带有细菌致癌质粒DF13(Clo DF13)的大肠杆菌小细胞中纯化酸性蛋白(分子量约为10,000),该蛋白可防止泄殖腔DF13抑制体外蛋白合成。事实证明,该蛋白质是在小细胞中由非诱导的Clo DF13质粒合成的三种Clo DF13质粒特异性多肽之一。此外,我们观察到,丝裂霉素C诱导后,免疫蛋白的量仅略有增加,而cloacin DF13的合成增加了约40倍。这些结果表明,编码免疫蛋白和cloacin DF13的基因不在同一调节单元中。在非诱导条件下,显然合成了过量的免疫蛋白,因为该量的免疫蛋白甚至足以中和诱导后显着增加的cloacin量,因为诱导的cloacinogenic细胞继续生长。

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