Quantitative Phosphoproteomics Reveal mTORC1 Activates de Novo Pyrimidine Synthesis

Aaron M. Robitaille; Stefan Christen; Mitsugu Shimobayashi; Marion Cornu; Luca L. Fava; Suzette Moes; Cristina Prescianotto‐Baschong; Uwe Sauer; Paul Jenoe; Michael N. Hall

doi:10.1126/science.1228771

Quantitative Phosphoproteomics Reveal mTORC1 Activates de Novo Pyrimidine Synthesis

Aaron M. Robitaille(University of Basel), Stefan Christen(Board of the Swiss Federal Institutes of Technology), Mitsugu Shimobayashi(University of Basel), Marion Cornu(University of Basel), Luca L. Fava(University of Basel), Suzette Moes(University of Basel), Cristina Prescianotto‐Baschong(University of Basel), Uwe Sauer(Board of the Swiss Federal Institutes of Technology), Paul Jenoe(University of Basel), Michael N. Hall(University of Basel)

Science

February 22, 2013

10.1126/science.1228771

Cited by 521

Abstract

The Ser-Thr kinase mammalian target of rapamycin (mTOR) controls cell growth and metabolism by stimulating glycolysis and synthesis of proteins and lipids. To further understand the central role of mTOR in cell physiology, we used quantitative phosphoproteomics to identify substrates or downstream effectors of the two mTOR complexes. mTOR controlled the phosphorylation of 335 proteins, including CAD (carbamoyl-phosphate synthetase 2, aspartate transcarbamylase, and dihydroorotase). CAD catalyzes the first three steps in de novo pyrimidine synthesis. mTORC1 indirectly phosphorylated CAD-S1859 through S6 kinase (S6K). CAD-S1859 phosphorylation promoted CAD oligomerization and thereby stimulated de novo synthesis of pyrimidines and progression through S phase of the cell cycle in mammalian cells. Thus, mTORC1 also stimulates the synthesis of nucleotides to control cell proliferation.

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