Control of septum thickness by the curvature of SepF polymers

Author:

Wenzel MichaelaORCID,Celik Gulsoy Ilkay N.,Gao Yongqiang,Teng Zihao,Willemse Joost,Middelkamp MartijnORCID,van Rosmalen Mariska G. M.ORCID,Larsen Per W. B.,van der Wel Nicole N.ORCID,Wuite Gijs J. L.,Roos Wouter H.,Hamoen Leendert W.ORCID

Abstract

Gram-positive bacteria divide by forming a thick cross wall. How the thickness of this septal wall is controlled is unknown. In this type of bacteria, the key cell division protein FtsZ is anchored to the cell membrane by two proteins, FtsA and/or SepF. We have isolated SepF homologs from different bacterial species and found that they all polymerize into large protein rings with diameters varying from 19 to 44 nm. Interestingly, these values correlated well with the thickness of their septa. To test whether ring diameter determines septal thickness, we tried to construct different SepF chimeras with the purpose to manipulate the diameter of the SepF protein ring. This was indeed possible and confirmed that the conserved core domain of SepF regulates ring diameter. Importantly, when SepF chimeras with different diameters were expressed in the bacterial hostBacillus subtilis, the thickness of its septa changed accordingly. These results strongly support a model in which septal thickness is controlled by curved molecular clamps formed by SepF polymers attached to the leading edge of nascent septa. This also implies that the intrinsic shape of a protein polymer can function as a mold to shape the cell wall.

Funder

Nederlandse Organisatie voor Wetenschappelijk Onderzoek

Electron Microscopy Center Amsterdam

NWO | Stichting voor de Technische Wetenschappen

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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