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Imaging of Streptomyces coelicolor A3(2) with Reduced Autofluorescence Reveals a Novel Stage of FtsZ Localization

机译:减少自身荧光的链霉菌coelicolor A3(2)的成像揭示了FtsZ定位的新阶段。

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摘要

Imaging of low abundance proteins in time and space by fluorescence microscopy is typically hampered by host-cell autofluorescence. Streptomycetes are an important model system for the study of bacterial development, and undergo multiple synchronous cell division during the sporulation stage. To analyse this phenomenon in detail, fluorescence microscopy, and in particular also the recently published novel live imaging techniques, require optimal signal to noise ratios. Here we describe the development of a novel derivative of Streptomyces coelicolor A3(2) with strongly reduced autofluorescence, allowing the imaging of fluorescently labelled proteins at significantly higher resolution. The enhanced image detail provided novel localization information for the cell division protein FtsZ, demonstrating a new developmental stage where multiple FtsZ foci accumulate at the septal plane. This suggests that multiple foci are sequentially produced, ultimately connecting to form the complete Z ring. The enhanced imaging properties are an important step forward for the confocal and live imaging of less abundant proteins and for the use of lower intensity fluorophores in streptomycetes.
机译:通过荧光显微镜在时间和空间上对低丰度蛋白质的成像通常会受到宿主细胞自发荧光的阻碍。链霉菌是研究细菌发育的重要模型系统,在孢子形成阶段经历多个同步细胞分裂。为了详细分析这种现象,荧光显微镜,尤其是最近发表的新颖的实时成像技术,要求最佳的信噪比。在这里,我们描述了一种新的Streptomyces coelicolor A3(2)衍生物的发展,该衍生物具有显着降低的自发荧光,可以显着更高的分辨率成像荧光标记的蛋白质。增强的图像细节为细胞分裂蛋白FtsZ提供了新颖的定位信息,展示了一个新的发育阶段,其中多个FtsZ病灶聚集在间隔平面上。这表明依次产生多个病灶,最终连接形成完整的Z环。对于低丰度蛋白质的共聚焦和实时成像以及在链霉菌中使用较低强度的荧光团,增强的成像性能是重要的一步。

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