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Inducible Expression of spo0A as a Universal Tool for Studying Sporulation in Clostridium difficile

机译:spo0A的诱导表达作为研究艰难梭菌孢子形成的通用工具

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摘要

Clostridium difficile remains a leading nosocomial pathogen, putting considerable strain on the healthcare system. The ability to form endospores, highly resistant to environmental insults, is key to its persistence and transmission. However, important differences exist between the sporulation pathways of C. difficile and the model Gram-positive organism Bacillus subtilis. Amongst the challenges in studying sporulation in C. difficile is the relatively poor levels of sporulation and high heterogeneity in the sporulation process. To overcome these limitations we placed Ptet regulatory elements upstream of the master regulator of sporulation, spo0A, generating a new strain that can be artificially induced to sporulate by addition of anhydrotetracycline (ATc). We demonstrate that this strain is asporogenous in the absence of ATc, and that ATc can be used to drive faster and more efficient sporulation. Induction of Spo0A is titratable and this can be used in the study of the spo0A regulon both in vitro and in vivo, as demonstrated using a mouse model of C. difficile infection (CDI). Insights into differences between the sporulation pathways in B. subtilis and C. difficile gained by study of the inducible strain are discussed, further highlighting the universal interest of this tool. The Ptet-spo0A strain provides a useful background in which to generate mutations in genes involved in sporulation, therefore providing an exciting new tool to unravel key aspects of sporulation in C. difficile.
机译:艰难梭菌仍然是主要的医院病原体,给医疗保健系统带来了很大压力。形成对环境污染具有高度抵抗力的内生孢子的能力是其持久性和传播的关键。但是,艰难梭菌的孢子形成途径与模型革兰氏阳性生物枯草芽孢杆菌之间存在重要差异。研究艰难梭菌孢子形成的挑战之一是相对较低的孢子形成水平和较高的异质性。为了克服这些局限性,我们将Ptet调控元件置于孢子形成的主要调控因子spo0A的上游,产生一种新菌株,可以通过添加脱水四环素(ATc)人工诱导使其形成孢子。我们证明,在没有ATc的情况下,该菌株是产孢子的,并且ATc可用于驱动更快,更有效的孢子形成。 Spo0A的诱导是可滴定的,可用于体外和体内Spo0A调节剂的研究,如使用艰难梭菌感染小鼠模型(CDI)所证实的。讨论了通过研究诱导型菌株获得的枯草芽孢杆菌和艰难梭菌孢子形成途径之间差异的见解,进一步凸显了该工具的普遍兴趣。 Ptet-spo0A菌株提供了有用的背景,可在其中产生与孢子形成有关的基因突变,因此提供了一种令人兴奋的新工具,可用于阐明艰难梭菌的孢子形成的关键方面。

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