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A single-step method for purification of active His-tagged ribosomes from a genetically engineered Escherichia coli

机译:一种从基因工程大肠杆菌中纯化具有活性的带His标签的核糖体的一步法

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摘要

With the rapid development of the ribosome field in recent years a quick, simple and high-throughput method for purification of the bacterial ribosome is in demand. We have designed a new strain of Escherichia coli (JE28) by an in-frame fusion of a nucleotide sequence encoding a hexa-histidine affinity tag at the 3′-end of the single copy rplL gene (encoding the ribosomal protein L12) at the chromosomal site of the wild-type strain MG1655. As a result, JE28 produces a homogeneous population of ribosomes (His)6-tagged at the C-termini of all four L12 proteins. Furthermore, we have developed a single-step, high-throughput method for purification of tetra-(His)6-tagged 70S ribosomes from this strain using affinity chromatography. These ribosomes, when compared with the conventionally purified ones in sucrose gradient centrifugation, 2D-gel, dipeptide formation and a full-length protein synthesis assay showed higher yield and activity. We further describe how this method can be adapted for purification of ribosomal subunits and mutant ribosomes. These methodologies could, in principle, also be used to purify any functional multimeric complex from the bacterial cell.
机译:随着近年来核糖体领域的快速发展,需要一种快速,简单和高通量的细菌核糖体纯化方法。我们通过在单拷贝rplL基因(编码核糖体蛋白L12)的3'端编码六组氨酸亲和标签的核苷酸序列进行框内融合,设计了一种新的大肠杆菌(JE28)菌株。野生型菌株MG1655的染色体位点。结果,JE28在所有四个L12蛋白的C末端产生了均一的核糖体(His)6-tagged标记。此外,我们已经开发出一种单步,高通量的方法,使用亲和色谱法从该菌株中纯化带有四(His)6标签的70S核糖体。与在蔗糖梯度离心,2D凝胶,二肽形成和全长蛋白质合成测定中常规纯化的核糖体相比,这些核糖体显示出更高的产率和活性。我们进一步描述了该方法如何适用于纯化核糖体亚基和突变核糖体。这些方法原则上也可以用于从细菌细胞中纯化任何功能性多聚体复合物。

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