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使用细胞分选和自动门控技术定量和分离枯草芽孢杆菌孢子。

Quantification and isolation of Bacillus subtilis spores using cell sorting and automated gating.

机构信息

Computer-aided Synthetic Biology, Institute for Biology, Technische Universität Darmstadt, Darmstadt, Germany.

出版信息

PLoS One. 2019 Jul 29;14(7):e0219892. doi: 10.1371/journal.pone.0219892. eCollection 2019.

Abstract

The Gram-positive bacterium Bacillus subtilis is able to form endospores which have a variety of biotechnological applications. Due to this ability, B. subtilis is as well a model organism for cellular differentiation processes. Sporulating cultures of B. subtilis form sub-populations which include vegetative cells, sporulating cells and spores. In order to readily and rapidly quantify spore formation we employed flow cytometric and fluorescence activated cell sorting techniques in combination with nucleic acid fluorescent staining in order to investigate the distribution of sporulating cultures on a single cell level. Automated gating procedures using Gaussian mixture modeling (GMM) were employed to avoid subjective gating and allow for the simultaneous measurement of controls. We utilized the presented method for monitoring sporulation over time in germination deficient strains harboring different genome modifications. A decrease in the sporulation efficiency of strain Bs02018, utilized for the display of sfGFP on the spores surface was observed. On the contrary, a double knock-out mutant of the phosphatase gene encoding Spo0E and of the spore killing factor SkfA (Bs02025) exhibited the highest sporulation efficiency, as within 24 h of cultivation in sporulation medium, cultures of BS02025 already consisted of 80% spores as opposed to 18% for the control strain. We confirmed the identity of the different subpopulations formed during sporulation by employing sorting and microscopy.

摘要

革兰氏阳性细菌枯草芽孢杆菌能够形成芽孢,这些芽孢具有多种生物技术应用。由于这种能力,枯草芽孢杆菌也是细胞分化过程的模式生物。形成芽孢的枯草芽孢杆菌培养物形成了包括营养细胞、芽孢形成细胞和芽孢的亚群。为了方便、快速地定量形成的芽孢,我们采用了流式细胞术和荧光激活细胞分选技术,并结合核酸荧光染色,以便在单细胞水平上研究芽孢形成培养物的分布。使用高斯混合模型(GMM)的自动门控程序被用来避免主观门控,并允许同时测量对照。我们利用该方法监测不同基因组修饰的发芽缺陷菌株中随时间的芽孢形成。观察到表面展示 sfGFP 的菌株 Bs02018 的芽孢形成效率降低。相反,编码 Spo0E 的磷酸酶基因和孢子杀伤因子 SkfA 的双敲除突变体 Bs02025 表现出最高的芽孢形成效率,因为在芽孢形成培养基中培养 24 小时后,BS02025 培养物中已经有 80%的芽孢,而对照菌株仅为 18%。我们通过分选和显微镜确认了在芽孢形成过程中形成的不同亚群的身份。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cf3d/6663000/b15ef3426d2c/pone.0219892.g001.jpg

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