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Use of targetrons to disrupt essential and nonessential genes in Staphylococcus aureus reveals temperature sensitivity of Ll.LtrB group II intron splicing

机译:使用靶标破坏金黄色葡萄球菌中的必需基因和非必需基因揭示了Ll.LtrB II组内含子剪接的温度敏感性

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摘要

We show that a targetron based on the Lactococcus lactis Ll.LtrB group II intron can be used for efficient chromosomal gene disruption in the human pathogen Staphylococcus aureus. Targetrons expressed from derivatives of vector pCN37, which uses a cadmium-inducible promoter, or pCN39, a derivative of pCN37 with a temperature-sensitive replicon, gave site-specific disruptants of the hsa and seb genes in 37%–100% of plated colonies without selection. To disrupt hsa, an essential gene, we used a group II intron that integrates in the sense orientation relative to target gene transcription and thus could be removed by RNA splicing, enabling the production of functional HSa protein. We show that because splicing of the Ll.LtrB intron by the intron-encoded protein is temperature-sensitive, this method yields a conditional hsa disruptant that grows at 32°C but not 43°C. The temperature sensitivity of the splicing reaction suggests a general means of obtaining one-step conditional disruptions in any organism. In nature, temperature sensitivity of group II intron splicing could limit the temperature range of an organism containing a group II intron inserted in an essential gene.
机译:我们表明基于乳酸乳球菌Ll.LtrB组II内含子的靶标可以用于人类病原体金黄色葡萄球菌的有效染色体基因破坏。由载体pCN37的衍生物表达的靶标,该载体使用镉诱导的启动子,或pCN39是具有温度敏感性复制子的pCN37的衍生物,可在37%–100%的平板菌落中产生hsa和seb基因的位点特异性破坏子。没有选择。为了破坏必需基因hsa,我们使用了II组内含子,该内含子以相对于靶基因转录的有义方向整合,因此可以通过RNA剪接除去,从而能够产生功能性HSa蛋白。我们表明,由于内含子编码蛋白对L.LtrB内含子的剪接是温度敏感的,因此该方法产生的条件性hsa破坏物在32°C而不是43°C时生长。剪接反应的温度敏感性表明,在任何生物中获得一步式条件性破坏的一般方法。实际上,II组内含子剪接的温度敏感性可能会限制插入必需基因中包含II组内含子的生物的温度范围。

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