AI Article Synopsis

  • Bacillus subtilis is effective at producing enzymes and biopharmaceuticals, but its extracellular proteases can degrade these proteins, limiting its use as a protein production system.
  • Genetic and chemical methods have been used to reduce protease activity, yet their effects had not been systematically compared until this study.
  • The research found that genetic inhibition of proteases is generally more effective in minimizing protein degradation, but chemical inhibitors can still enhance production of sensitive proteins in certain mutant strains.

Article Abstract

Bacillus subtilis is a prolific producer of enzymes and biopharmaceuticals. However, the susceptibility of heterologous proteins to degradation by (extracellular) proteases is a major limitation for use of B. subtilis as a protein cell factory. An increase in protein production levels has previously been achieved by using either protease-deficient strains or addition of protease inhibitors to B. subtilis cultures. Notably, the effects of genetic and chemical inhibition of proteases have thus far not been compared in a systematic way. In the present studies, we therefore compared the exoproteomes of cells in which extracellular proteases were genetically or chemically inactivated. The results show substantial differences in the relative abundance of various extracellular proteins. Furthermore, a comparison of the effects of genetic and/or chemical protease inhibition on the stress response triggered by (over) production of secreted proteins showed that chemical protease inhibition provoked a genuine secretion stress response. From a physiological point of view, this suggests that the deletion of protease genes is a better way to prevent product degradation than the use of protease inhibitors. Importantly however, studies with human interleukin-3 show that chemical protease inhibition can result in improved production of protease-sensitive secreted proteins even in mutant strains lacking eight extracellular proteases.

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Source
http://dx.doi.org/10.1002/pmic.200800009DOI Listing

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