Periodic Reporting for period 4 - STRINGENCY (Control of Bacterial Multidrug Tolerance and Stress Response by Alarmone Synthetase SpoT)
Berichtszeitraum: 2021-07-01 bis 2021-12-31
The Stringent Response is a general bacterial stress response induced by diverse nutritional and environmental stresses allowing bacteria to adapt and survive adverse conditions. This global resetting of bacterial cells physiology relies on the accumulation of two unusual phosphorylated derivatives of GTP and GDP collectively called (p)ppGpp which are synthetized by the RelA/SpoT homologue proteins. Importantly the Stringent Response has a key role in bacterial virulence and in the formation of antibiotic-tolerant cells. However, the molecular mechanisms by which environmental cues activate the stringent response are still largely unknown and represent one of the most fundamental, unsolved problems in prokaryotic molecular biology. Thus, there is a pressing need to understand how the activities of the enzymes responsible for synthesis and degradation of (p)ppGpp are regulated and to develop novel strategies to combat recalcitrant infections. Therefore, the STRINGENCY project aims to uncover the molecular mechanisms by which environmental stimuli trigger SpoT-dependent (p)ppGpp synthesis with special emphasis on its role in the formation of multidrug tolerant cells in Escherichia coli. The STRINGENCY project was organized around three main objectives: (i) To unravel how spoT expression is regulated (ii) To reveal how (p)ppGpp synthetase II activity encoded by spoT is mechanistically controlled and (iii) To decipher the physiological role of SpoT in multidrug tolerance. The results of this ambitious research program have significantly improved our understanding of (p)ppGpp biology and its impact on bacterial cell physiology.
To gain further insights into the regulation of the bifunctional (p)ppGpp synthetase/hydrolase SpoT enzyme we have successfully developed genetic assays that allowed us to identify new protein candidates that modulate (p)ppGpp level in E. coli. We have isolated six candidates that either promotes accumulation or degradation of (p)ppGpp in vivo.
Among them we observed that YtfK, a small protein of unknown function, is required to sustain elevated (p)ppGpp levels in response to phosphate, carbon and fatty acid starvation, therefore ensuring cell survival under these stress conditions. Interestingly YtfK is also needed to produce antibiotic tolerant cells under nutritional stress conditions, further highlighting the important role of SpoT and the signaling molecule (p)ppGpp in controlling multidrug tolerance. Mechanistically we show that YtfK controls the stringent response via a direct and specific interaction with the N-terminal region of SpoT encompassing the hydrolase and synthetase domains. We further observed that YtfK modifies the protein surface of SpoT catalytic domains supporting conformational changes upon binding and suggesting that YtfK acts by tilting the catalytic balance of SpoT toward (p)ppGpp synthesis rather than hydrolysis. In addition we decipher the genetic controls involved in the regulation of ytfK expression and its impact on the cell physiology. We observed that ytfK is subjected to catabolite repression and is positively regulated by the cyclic AMP (cAMP)-cAMP receptor protein (CRP) complex. Moreover we observed that YtfK controls SpoT-dependent accumulation of (p)ppGpp, cell survival and formation of antibiotic tolerant cells in response to carbon starvation.
Finally we uncovered an unprecedented mode of regulation that inhibits the stringent response in Escherichia coli. Indeed, we discovered that the small subunit of the nitrite reductase NirD prevents (p)ppGpp accumulation in vivo from the mono-functional (p)ppGpp synthetase RelA. Remarkably, NirD modulates the stringent response by direct binding to RelA in vivo. Mechanistically, our in vitro results show that binding of NirD to the catalytic domains of RelA directly inhibits the rate of pppGpp synthesis.
Taken together, the identification of new partners that modulate the stringent response and the characterization of the molecular mechanisms behind these regulations have critically increase our knowledge of (p)ppGpp biology and bacterial survival mechanisms and may, in the future, improve biotechnological processes and how bacterial infections are treated
Among them we observed that YtfK, a small protein of unknown function, is required to sustain elevated (p)ppGpp levels in response to phosphate, carbon and fatty acid starvation, therefore ensuring cell survival under these stress conditions. Interestingly YtfK is also needed to produce antibiotic tolerant cells under nutritional stress conditions, further highlighting the important role of SpoT and the signaling molecule (p)ppGpp in controlling multidrug tolerance. Mechanistically we show that YtfK controls the stringent response via a direct and specific interaction with the N-terminal region of SpoT encompassing the hydrolase and synthetase domains. We further observed that YtfK modifies the protein surface of SpoT catalytic domains supporting conformational changes upon binding and suggesting that YtfK acts by tilting the catalytic balance of SpoT toward (p)ppGpp synthesis rather than hydrolysis. In addition we decipher the genetic controls involved in the regulation of ytfK expression and its impact on the cell physiology. We observed that ytfK is subjected to catabolite repression and is positively regulated by the cyclic AMP (cAMP)-cAMP receptor protein (CRP) complex. Moreover we observed that YtfK controls SpoT-dependent accumulation of (p)ppGpp, cell survival and formation of antibiotic tolerant cells in response to carbon starvation.
Finally we uncovered an unprecedented mode of regulation that inhibits the stringent response in Escherichia coli. Indeed, we discovered that the small subunit of the nitrite reductase NirD prevents (p)ppGpp accumulation in vivo from the mono-functional (p)ppGpp synthetase RelA. Remarkably, NirD modulates the stringent response by direct binding to RelA in vivo. Mechanistically, our in vitro results show that binding of NirD to the catalytic domains of RelA directly inhibits the rate of pppGpp synthesis.
Taken together, the identification of new partners that modulate the stringent response and the characterization of the molecular mechanisms behind these regulations have critically increase our knowledge of (p)ppGpp biology and bacterial survival mechanisms and may, in the future, improve biotechnological processes and how bacterial infections are treated
The stringent response has been investigated for more than 50 years. Therefore, identification and the characterization of new protein partners that modulates (p)ppGpp represent important conceptual advances in the understanding of bacterial stress response and cell survival mechanisms. Therefore the STRINGENCY project has pushed forward our understanding of the molecular mechanisms underlying the stringent response and we anticipate that it will open new perspectives for the development of novel drug-target discovery regimes to fight recurrent infections.