Open Access
How the initiating ribosome copes with ppGpp to translate mRNAs
Daria V. Vinogradova
1
,
Victor Zegarra
2
,
Elena Maksimova
3
,
Jose A Nakamoto
2
,
Pavel Kasatsky
3
,
Alena Paleskava
1
,
Pohl Milón
2
1
2
Centre for Research and Innovation, Faculty of Health Sciences, Universidad Peruana de Ciencias Aplicadas (UPC), Lima, Peru
|
Publication type: Journal Article
Publication date: 2020-01-29
scimago Q1
wos Q1
SJR: 2.691
CiteScore: 10.3
Impact factor: 7.2
ISSN: 15449173, 15457885
PubMed ID:
31995552
General Biochemistry, Genetics and Molecular Biology
General Agricultural and Biological Sciences
General Immunology and Microbiology
General Neuroscience
Abstract
During host colonization, bacteria use the alarmones (p)ppGpp to reshape their proteome by acting pleiotropically on DNA, RNA, and protein synthesis. Here, we elucidate how the initiating ribosome senses the cellular pool of guanosine nucleotides and regulates the progression towards protein synthesis. Our results show that the affinity of guanosine triphosphate (GTP) and the inhibitory concentration of ppGpp for the 30S-bound initiation factor IF2 vary depending on the programmed mRNA. The TufA mRNA enhanced GTP affinity for 30S complexes, resulting in improved ppGpp tolerance and allowing efficient protein synthesis. Conversely, the InfA mRNA allowed ppGpp to compete with GTP for IF2, thus stalling 30S complexes. Structural modeling and biochemical analysis of the TufA mRNA unveiled a structured enhancer of translation initiation (SETI) composed of two consecutive hairpins proximal to the translation initiation region (TIR) that largely account for ppGpp tolerance under physiological concentrations of guanosine nucleotides. Furthermore, our results show that the mechanism enhancing ppGpp tolerance is not restricted to the TufA mRNA, as similar ppGpp tolerance was found for the SETI-containing Rnr mRNA. Finally, we show that IF2 can use pppGpp to promote the formation of 30S initiation complexes (ICs), albeit requiring higher factor concentration and resulting in slower transitions to translation elongation. Altogether, our data unveil a novel regulatory mechanism at the onset of protein synthesis that tolerates physiological concentrations of ppGpp and that bacteria can exploit to modulate their proteome as a function of the nutritional shift happening during stringent response and infection.
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Vinogradova D. V. et al. How the initiating ribosome copes with ppGpp to translate mRNAs // PLoS Biology. 2020. Vol. 18. No. 1. p. e3000593.
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Vinogradova D. V., Zegarra V., Maksimova E., Nakamoto J. A., Kasatsky P., Paleskava A., Konevega A. L., Milón P. How the initiating ribosome copes with ppGpp to translate mRNAs // PLoS Biology. 2020. Vol. 18. No. 1. p. e3000593.
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RIS
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TY - JOUR
DO - 10.1371/journal.pbio.3000593
UR - https://dx.plos.org/10.1371/journal.pbio.3000593
TI - How the initiating ribosome copes with ppGpp to translate mRNAs
T2 - PLoS Biology
AU - Vinogradova, Daria V.
AU - Zegarra, Victor
AU - Maksimova, Elena
AU - Nakamoto, Jose A
AU - Kasatsky, Pavel
AU - Paleskava, Alena
AU - Konevega, Andrey L.
AU - Milón, Pohl
PY - 2020
DA - 2020/01/29
PB - Public Library of Science (PLoS)
SP - e3000593
IS - 1
VL - 18
PMID - 31995552
SN - 1544-9173
SN - 1545-7885
ER -
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BibTex (up to 50 authors)
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@article{2020_Vinogradova,
author = {Daria V. Vinogradova and Victor Zegarra and Elena Maksimova and Jose A Nakamoto and Pavel Kasatsky and Alena Paleskava and Andrey L. Konevega and Pohl Milón},
title = {How the initiating ribosome copes with ppGpp to translate mRNAs},
journal = {PLoS Biology},
year = {2020},
volume = {18},
publisher = {Public Library of Science (PLoS)},
month = {jan},
url = {https://dx.plos.org/10.1371/journal.pbio.3000593},
number = {1},
pages = {e3000593},
doi = {10.1371/journal.pbio.3000593}
}
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MLA
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Vinogradova, Daria V., et al. “How the initiating ribosome copes with ppGpp to translate mRNAs.” PLoS Biology, vol. 18, no. 1, Jan. 2020, p. e3000593. https://dx.plos.org/10.1371/journal.pbio.3000593.