AI Article Synopsis

  • Serovar L2 (Ct) divides through a unique polarized budding process instead of traditional binary fission, due to its lack of FtsZ, a protein common in other bacteria.
  • The assembly of the divisome, essential for cell division, is initiated by FtsK, which forms specific focal points at the site where new daughter cells will emerge, signifying its role in the division process.
  • Research indicates that FtsK is crucial for recruiting other proteins to the divisome, while MreB, though necessary for forming peptidoglycan rings, does not serve as the primary scaffold for divisome assembly.

Article Abstract

serovar L2 (Ct), an obligate intracellular bacterium that does not encode FtsZ, divides by a polarized budding process. In the absence of FtsZ, we show that divisome assembly in is initiated by FtsK, a chromosomal translocase. Chlamydial FtsK forms discrete foci at the septum and at the base of the progenitor mother cell, and our data indicate that FtsK foci at the base of the mother cell mark the location of nascent divisome complexes that form at the site where a daughter cell will emerge in the next round of division. The divisome in has a hybrid composition, containing elements of the divisome and elongasome from other bacteria, and FtsK is recruited to nascent divisomes prior to the other chlamydial divisome proteins assayed, including the PBP2 and PBP3 transpeptidases, and MreB and MreC. Knocking down FtsK prevents divisome assembly in and inhibits cell division and septal peptidoglycan synthesis. We further show that MreB does not function like FtsZ and serve as a scaffold for the assembly of the divisome. Rather, MreB is one of the last proteins recruited to the chlamydial divisome, and it is necessary for the formation of septal peptidoglycan rings. Our studies illustrate the critical function of chlamydial FtsK in coordinating divisome assembly and peptidoglycan synthesis in this obligate intracellular bacterial pathogen.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11527202PMC
http://dx.doi.org/10.1101/2024.10.24.620021DOI Listing

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