Migration of Polyphosphate Granules in Agrobacterium tumefaciens.

Pub Date : 2022-01-01 Epub Date: 2022-02-15 DOI:10.1159/000521970
Celina Frank, Daniel Pfeiffer, Meriyem Aktas, Dieter Jendrossek
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引用次数: 3

Abstract

Agrobacterium tumefaciens has two polyphosphate (polyP) kinases, one of which (PPK1AT) is responsible for the formation of polyP granules, while the other (PPK2AT) is used for replenishing the NTP pools by using polyP as a phosphate donor to phosphorylate nucleoside diphosphates. Fusions of eYFP with PPK2AT or of the polyP granule-associated phosin PptA from Ralstonia eutropha always co-localized with polyP granules in A. tumefaciens and allowed the tracking of polyP granules in time-lapse microscopy experiments without the necessity to label the cells with the toxic dye DAPI. Fusions of PPK1AT with mCherry formed fluorescent signals often attached to, but not completely co-localizing with, polyP granules in wild-type cells. Time-lapse microscopy revealed that polyP granules in about one-third of a cell population migrated from the old pole to the new cell pole shortly before or during cell division. Many cells de novo formed a second (nonmigrating) polyP granule at the opposite cell pole before cell division was completed, resulting in two daughter cells each having a polyP granule at the old pole after septum formation. Migration of polyP granules was disordered in mitomycin C-treated or in PopZ-depleted cells, suggesting that polyP granules can associate with DNA or with other molecules that are segregated during the cell cycle.

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农杆菌中多磷酸盐颗粒的迁移。
根癌农杆菌有两种多磷酸(polyP)激酶,其中一种(PPK1AT)负责polyP颗粒的形成,而另一种(PPK2AT)通过使用polyP作为磷酸盐供体磷酸化核苷二磷酸来补充NTP库。eYFP与PPK2AT或富营养Ralstonia polyP颗粒相关phosin PptA的融合总是与A. memefaciens中的息肉颗粒共定位,并且允许在延迟显微镜实验中跟踪息肉颗粒,而无需用有毒染料DAPI标记细胞。在野生型细胞中,PPK1AT与mCherry融合形成的荧光信号通常附着在息肉颗粒上,但不完全与息肉颗粒共定位。延时显微镜显示,大约三分之一的细胞群中的息肉颗粒在细胞分裂前不久或分裂期间从旧细胞极迁移到新细胞极。许多细胞在细胞分裂完成之前在相反的细胞极形成第二个(非迁移的)息肉颗粒,导致两个子细胞在隔形成后的旧极各有一个息肉颗粒。在丝裂霉素c处理或popz缺失的细胞中,息肉颗粒的迁移被扰乱,这表明息肉颗粒可以与DNA或细胞周期中分离的其他分子结合。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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