AI Article Synopsis

  • Proteolysis is vital for regulating protein levels and functions across all living organisms, with the Lon protease in E. coli playing a key role in protein quality control.
  • A quantitative Super-SILAC mass spectrometry technique was used to compare the proteomes of a lon mutant and a Lon-producing strain, leading to the identification of 14 new Lon substrates.
  • The findings also highlighted Lon's involvement in various processes, including superoxide stress response, sulfur assimilation, nucleotide biosynthesis, and central energy metabolism.

Article Abstract

Controlling the cellular abundance and proper function of proteins by proteolysis is a universal process in all living organisms. In Escherichia coli, the ATP-dependent Lon protease is crucial for protein quality control and regulatory processes. To understand how diverse substrates are selected and degraded, unbiased global approaches are needed. We employed a quantitative Super-SILAC (stable isotope labeling with amino acids in cell culture) mass spectrometry approach and compared the proteomes of a lon mutant and a strain producing the protease to discover Lon-dependent physiological functions. To identify Lon substrates, we took advantage of a Lon trapping variant, which is able to translocate substrates but unable to degrade them. Lon-associated proteins were identified by label-free LC-MS/MS. The combination of both approaches revealed a total of 14 novel Lon substrates. Besides the identification of known pathways affected by Lon, for example, the superoxide stress response, our cumulative data suggests previously unrecognized fundamental functions of Lon in sulfur assimilation, nucleotide biosynthesis, amino acid and central energy metabolism.

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Source
http://dx.doi.org/10.1002/pmic.201800080DOI Listing

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