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通过对固定细胞的单分子定位显微镜观察,获得大肠杆菌细胞分裂过程中FtsZ重排的新见解。

New insights into FtsZ rearrangements during the cell division of Escherichia coli from single-molecule localization microscopy of fixed cells.

作者信息

Vedyaykin Alexey D, Vishnyakov Innokentii E, Polinovskaya Vasilisa S, Khodorkovskii Mikhail A, Sabantsev Anton V

机构信息

Institute of Nanobiotechnologies, Peter the Great St. Petersburg Polytechnic University, Polytechnicheskaya str. 29, Saint Petersburg, 195251, Russia.

Institute of Cytology, Russian Academy of Sciences, Tikhoretsky av. 4, Saint Petersburg, 194064, Russia.

出版信息

Microbiologyopen. 2016 Jun;5(3):378-86. doi: 10.1002/mbo3.336. Epub 2016 Feb 3.

Abstract

FtsZ - a prokaryotic tubulin homolog - is one of the central components of bacterial division machinery. At the early stage of cytokinesis FtsZ forms the so-called Z-ring at mid-cell that guides septum formation. Many approaches were used to resolve the structure of the Z-ring, however, researchers are still far from consensus on this question. We utilized single-molecule localization microscopy (SMLM) in combination with immunofluorescence staining to visualize FtsZ in Esherichia coli fixed cells that were grown under slow and fast growth conditions. This approach allowed us to obtain images of FtsZ structures at different stages of cell division and accurately measure Z-ring dimensions. Analysis of these images demonstrated that Z-ring thickness increases during constriction, starting at about 70 nm at the beginning of division and increasing by approximately 25% half-way through constriction.

摘要

FtsZ(一种原核微管蛋白同源物)是细菌分裂机制的核心组成部分之一。在胞质分裂早期,FtsZ 在细胞中部形成所谓的Z环,引导隔膜形成。人们采用了多种方法来解析Z环的结构,然而,在这个问题上研究人员仍未达成共识。我们利用单分子定位显微镜(SMLM)结合免疫荧光染色,来观察在缓慢和快速生长条件下培养的大肠杆菌固定细胞中的FtsZ。这种方法使我们能够获得细胞分裂不同阶段FtsZ结构的图像,并准确测量Z环的尺寸。对这些图像的分析表明,Z环厚度在收缩过程中增加,在分裂开始时约为70纳米,在收缩到一半时增加约25%。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/af56/4905991/f960982989dc/MBO3-5-378-g001.jpg

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