AI Article Synopsis

  • Chromosome movement during mid-meiotic prophase is crucial for efficient homolog pairing and managing topological entanglements, particularly observed in budding yeast.
  • The research utilizes advanced 3D live-cell imaging with FROS labeling to analyze telomere movement, categorizing it into pauses, rapid transport, and slower directional motions influenced by actin dynamics.
  • Findings emphasize the significance of telomere movement and nuclear envelope deformations in chromosome organization, while the low-SNR imaging technique opens avenues for further studies on homolog pairing.

Article Abstract

Chromosome movement is prominent at mid-meiotic prophase and is proposed to enhance the efficiency and/or stringency of homolog pairing and/or to help prevent or resolve topological entanglements. Here, we combine fluorescent repressor operator system (FROS) labeling with three-dimensional (3D) live-cell imaging at high spatio-temporal resolution to define the detailed kinetics of mid-meiotic prophase motion for a single telomere-proximal locus in budding yeast. Telomere motions can be grouped into three general categories: (i) pauses, in which the telomere "jiggles in place"; (ii) rapid, straight/curvilinear motion which reflects Myo2/actin-mediated transport of the monitored telomere; and (iii) slower directional motions, most of which likely reflect indirectly promoted motion of the monitored telomere in coordination with actin-mediated motion of an unmarked telomere. These and other findings highlight the importance of dynamic assembly/disassembly of telomere/LINC/actin ensembles and also suggest important roles for nuclear envelope deformations promoted by actin-mediated telomere/LINC movement. The presented low-SNR (signal-to-noise ratio) imaging methodology provides opportunities for future exploration of homolog pairing and related phenomena.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8656277PMC
http://dx.doi.org/10.3389/fcell.2021.687132DOI Listing

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