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Highly Efficient and More General cis- and trans-Splicing Inteins through Sequential Directed Evolution

机译:通过有序定向进化的高效和更普遍的顺式和反式剪接蛋白

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摘要

Inteins are internal protein sequences that post-translationally self-excise and splice together the flanking sequences, the so-called exteins. Natural and engineered inteins have been used in many practical applications. However, inteins are often inefficient or inactive when placed in a non-native host protein and may require the presence of several amino acid residues of the native exteins, which will then remain as a potential scar in the spliced protein. Thus, more general inteins that overcome these limitations are highly desirable. Here we report sequential directed evolution as a new approach to produce inteins with such properties. Random mutants of the Ssp (Synechocystis sp. PCC 6803) DnaB mini-intein were inserted into the protein conferring kanamycin resistance at a site where the parent intein was inactive for splicing. The mutants selected for splicing activity were further improved by iterating the procedure for two more cycles at different positions in the same protein. The resulting improved inteins showed high activity in the positions of the first rounds of selection, in multiple new insertion sites, and in different proteins. One of these inteins, the M86 mutant, which accumulated 8 amino acid substitutions, was also biochemically characterized in an artificially split form with a chemically synthesized N-terminal intein fragment consisting of 11 amino acids. When compared with the unevolved split intein, it exhibited an ∼60-fold increased rate in the protein trans-splicing reaction and a Kd value for the interaction of the split intein fragments improved by an order of magnitude. Implications on the intein structure-function, practical application, and evolution are discussed.
机译:内含蛋白是内部蛋白质序列,其在翻译后自我消费并将侧翼序列(所谓的外在蛋白)拼接在一起。天然和工程化的内含肽已用于许多实际应用中。但是,内含蛋白在置于非天然宿主蛋白中时通常效率低下或失活,并且可能需要存在天然内在蛋白的多个氨基酸残基,然后这些残基将作为潜在的疤痕保留在剪接的蛋白中。因此,非常需要克服这些限制的更通用的内含子。在这里,我们报道了有序定向进化是生产具有这种特性的蛋白的新方法。将Ssp(Synechocystis sp。PCC 6803)DnaB mini-intein的随机突变体插入到赋予卡那霉素抗性的蛋白质中,其亲本intein对剪接没有活性。通过在相同蛋白质的不同位置重复两个循环以上的程序,进一步提高了选择用于剪接活性的突变体。所得的改进的内含肽在第一轮选择的位置,多个新的插入位点和不同的蛋白质中显示出高活性。这些内含蛋白之一,M86突变体,其积累了8个氨基酸取代,还以化学合成的由11个氨基酸组成的N末端内含蛋白片段以人工分裂的形式进行了生化表征。与未进化的分裂内含子相比,它在蛋白质反式分裂反应中的速率增加了约60倍,并且分裂内含蛋白片段相互作用的Kd值提高了一个数量级。讨论了对内含肽结构功能,实际应用和进化的影响。

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