AI Article Synopsis

  • PML nuclear bodies (NBs) play a crucial role in nuclear pathways, but their specific biochemical functions remain unclear.
  • The study utilized live cell imaging and mathematical modeling to assess the assembly dynamics of PML isoforms at NBs, revealing that they exhibit varied exchange rates and identifying PML V as a key scaffolding component.
  • Additionally, factors such as SUMOylation and ATP levels were found to influence the dynamics of protein turnover at NBs, paving the way for understanding the mechanisms involved in the targeting and regulation of proteins within these nuclear domains.

Article Abstract

PML nuclear bodies (NBs) are involved in the regulation of key nuclear pathways but their biochemical function in nuclear metabolism is unknown. In this study PML NB assembly dynamics were assessed by live cell imaging and mathematic modeling of its major component parts. We show that all six nuclear PML isoforms exhibit individual exchange rates at NBs and identify PML V as a scaffold subunit. SP100 exchanges at least five times faster at NBs than PML proteins. Turnover dynamics of PML and SP100 at NBs is modulated by SUMOylation. Exchange is not temperature-dependent but depletion of cellular ATP levels induces protein immobilization at NBs. The PML-RARalpha oncogene exhibits a strong NB retention effect on wild-type PML proteins. HIPK2 requires an active kinase for PML NB targeting and elevated levels of PML IV increase its residence time. DAXX and BLM turn over rapidly and completely at PML NBs within seconds. These findings provide a kinetics model for factor exchange at PML NBs and highlight potential mechanisms to regulate intranuclear trafficking of specific factors at these domains.

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Source
http://dx.doi.org/10.1242/jcs.031922DOI Listing

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