AI Article Synopsis

  • PPP-family phosphatases like PP1 lack intrinsic specificity and rely on cofactors such as Phactr1 to improve targeting to substrates and locations.
  • Phactr1, a regulator enriched in neurons and influenced by G-actin, alters PP1's structure by remodeling a hydrophobic groove near its catalytic site, enhancing its interaction with specific substrates.
  • The study identified specific substrates for Phactr1/PP1 through phosphoproteomics and demonstrated that sequence interactions with these substrates are essential for enhanced dephosphorylation efficiency compared to other forms of PP1.

Article Abstract

PPP-family phosphatases such as PP1 have little intrinsic specificity. Cofactors can target PP1 to substrates or subcellular locations, but it remains unclear how they might confer sequence-specificity on PP1. The cytoskeletal regulator Phactr1 is a neuronally enriched PP1 cofactor that is controlled by G-actin. Structural analysis showed that Phactr1 binding remodels PP1's hydrophobic groove, creating a new composite surface adjacent to the catalytic site. Using phosphoproteomics, we identified mouse fibroblast and neuronal Phactr1/PP1 substrates, which include cytoskeletal components and regulators. We determined high-resolution structures of Phactr1/PP1 bound to the dephosphorylated forms of its substrates IRSp53 and spectrin αII. Inversion of the phosphate in these holoenzyme-product complexes supports the proposed PPP-family catalytic mechanism. Substrate sequences C-terminal to the dephosphorylation site make intimate contacts with the composite Phactr1/PP1 surface, which are required for efficient dephosphorylation. Sequence specificity explains why Phactr1/PP1 exhibits orders-of-magnitude enhanced reactivity towards its substrates, compared to apo-PP1 or other PP1 holoenzymes.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7599070PMC
http://dx.doi.org/10.7554/eLife.61509DOI Listing

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