Ataxia-telangiectasia mutated (ATM) is a cellular damage sensor that coordinates the cell cycle with damage-response checkpoints and DNA repair to preserve genomic integrity. However, ATM also has been implicated in metabolic regulation, and ATM deficiency is associated with elevated reactive oxygen species (ROS). ROS has a central role in many physiological and pathophysiological processes including inflammation and chronic diseases such as atherosclerosis and cancer, underscoring the importance of cellular pathways involved in redox homeostasis. We have identified a cytoplasmic function for ATM that participates in the cellular damage response to ROS. We show that in response to elevated ROS, ATM activates the TSC2 tumor suppressor via the LKB1/AMPK metabolic pathway in the cytoplasm to repress mTORC1 and induce autophagy. Importantly, elevated ROS and dysregulation of mTORC1 in ATM-deficient cells is inhibited by rapamycin, which also rescues lymphomagenesis in Atm -deficient mice. Our results identify a cytoplasmic pathway for ROS-induced ATM activation of TSC2 to regulate mTORC1 signaling and autophagy, identifying an integration node for the cellular damage response with key pathways involved in metabolism, protein synthesis, and cell survival.
Loss of tuberin, the product of TSC2 gene, increases mammalian target of rapamycin (mTOR) signaling, promoting cell growth and tumor development. However, in cells expressing tuberin, it is not known how repression of mTOR signaling is relieved to activate this pathway in response to growth factors and how hamartin participates in this process. We show that hamartin colocalizes with hypophosphorylated tuberin at the membrane, where tuberin exerts its GTPase-activating protein (GAP) activity to repress Rheb signaling. In response to growth signals, tuberin is phosphorylated by AKT and translocates to the cytosol, relieving Rheb repression. Phosphorylation of tuberin at serines 939 and 981 does not alter its intrinsic GAP activity toward Rheb but partitions tuberin to the cytosol, where it is bound by 14-3-3 proteins. Thus, tuberin bound by 14-3-3 in response to AKT phosphorylation is sequestered away from its membrane-bound activation partner (hamartin) and its target GTPase (Rheb) to relieve the growth inhibitory effects of this tumor suppressor.
Is the Corrolate Macrocycle Innocent or Noninnocent? Magnetic Susceptibility, Mössbauer, 1H NMR, and DFT Investigations of Chloro- and Phenyliron Corrolates
In an attempt to determine the electron configuration of (anion)iron corrolates, i.e., whether they are S = 1 Fe(IV)-corrolate(3-) or S = 3/2 Fe(III)-corrolate(2-*), with antiferromagnetic coupling between the iron and macrocycle electrons to yield overall S = 1, two axial ligand complexes of an iron octaalkylcorrolate have been studied by temperature-dependent magnetic susceptibility, magnetic Mössbauer, and 1H NMR spectroscopy, and the results have been compared to those determined on the basis of spin-unrestricted DFT calculations. Magnetic susceptibility measurements indicate the presence of a noninnocent macrocycle (corrolate (2-*)) for the chloroiron corrolate, with strong antiferromagnetic coupling to the S = 3/2 Fe(III) center, while those for the phenyliron corrolate are not conclusive as to the electron configuration. Temperature- and field-dependent Mössbauer spectroscopic investigations of these two complexes yielded spectra that could be simulated with either electron configuration, except that the isomer shift of the phenyl-iron complex is -0.10 mm/s while that of the chloroiron complex is +0.21 mm/s, suggesting that the iron in the former is Fe(IV) while in the latter it is Fe(III). 1H NMR spectroscopic studies of both axial ligand complexes show large negative spin density at the meso carbons, with those of the chloroiron complex (Cai, S.; Walker, F. A.; Licoccia, S. Inorg. Chem. 2000, 39, 3466) being roughly four times larger than those of the phenyliron complex. The temperature dependence of the proton chemical shifts of the phenyliron complex is strictly linear. DFT calculations are consistent with the chloroiron complex being formulated as S1 = 3/2 Fe(III)-corrolate (2-*) S2 = 1/2, with negative spin density at all nitrogens and meso carbons, and a net spin density of -0.79 on the corrolate ring and positive spin density (+0.17) on the chloride ion and +2.58 on the iron. In contrast, the phenyliron complex is best formulated as S = 1 Fe(IV)-corrolate (3-), but again with negative spin density at all nitrogens and meso carbons of the macrocycle, yet with the net spin density on the corrolate ring being virtually zero; the phenyl carbanion carbon has relatively large negative spin density of -0.15 and the iron +2.05. On the basis of all of the results, we conclude that in both the chloroiron and phenyliron complexes the corrolate ring is noninnocent, in the chloroiron complex to a much larger extent than in the phenyliron complex.
Human and Escherichia coli derivatives of AlkB enzymes remove methyl groups from 1-methyladenine and 3-methylcytosine in nucleic acids via an oxidative mechanism that releases the methyl group as formaldehyde. In this report, we demonstrate that the mouse homologues of the ␣-ketoglutarate Fe(II) oxygen-dependent enzymes mAbh2 and Abh3 have activities comparable to those of their human counterparts. The mAbh2 and mAbh3 release modified bases from both DNA and RNA. Comparison of the activities of the homogenous ABH2 and ABH3 enzymes demonstrate that these activities are shared by both sets of enzymes. An assay for the detection of ␣-ketoglutarate Fe(II) dioxygenase activity using an oligodeoxyribonucleotide with a unique modification shows activity for all four enzymes studied and a loss of activity for eight mutant proteins. Steady-state kinetics for removal of methyl groups from DNA substrates indicates that the reactions of the proteins are close to the diffusion limit. Moreover, mAbh2 or mAbh3 activity increases survival in a strain defective in alkB. The mRNAs of AHB2 and ABH3 are expressed most in testis for ABH2 and ABH3, whereas expression of the homologous mouse genes is different. The mAbh3 is strongly expressed in testis, whereas highest expression of mAbh2 is in heart. Other purified human AlkB homologue proteins ABH4, ABH6, and ABH7 do not manifest activity. The demonstration of mAbh2 and mAbh3 activities and their distributions provide data on these mammalian homologues of AlkB that can be used in animal studies.Environmental and endogenous agents constantly subject DNA and RNA to damage. Alkylating agents cover a spectrum of chemicals that in their most simple form methylate DNA or RNA. The subsequent distribution of methylated products of the reaction of methylating agents with nucleic acids depends on the nature of the agent. S N 1 alkylating agents react via a carbonium ion intermediate whereas S N 2 agents interact directly with DNA (1). Under these circumstances different sites on nucleic acids are modified. In addition to the alkylating agent, the structure of the DNA also plays a role. Regions of single-stranded nucleic acids favor reaction at sites that are virtually untouched in doublestranded nucleic acids. For example, position 1 of Ade is not modified to any extent in double-stranded DNA (ds-DNA), 2 whereas in singlestranded DNA (ss-DNA) it becomes a major target (1-4).In 1983, an Escherichia coli mutant with sensitivity to S N 2 alkylating agents was isolated and named alkB (5). The cloning of the gene and the acknowledgment that it was linked to the ada operon responding to DNA alkylation damage produced enormous interest in this gene (6, 7). Despite the knowledge that expression of alkB in human cells could increase resistance to alkylating agents (8, 9), AlkB had no known enzymatic function. The genetic work in E. coli was important, but without function, progress in the line of AlkB lagged behind that of other DNA repair studies (10 -12). Even the isolation of a human homologue of A...
The chloroiron corrolates of 2,3,7,8,12,13,17,18-octamethyl- and 7,13-dimethyl-2,3,8,12,17,18-hexaethylcorrole ([(Me8C)FeCl] and [(7,13-Me2Et6C)FeCl], respectively) and their bisimidazole complexes have been investigated by NMR spectroscopy as a function of temperature, and by EPR spectroscopy at 4.2 K. Magnetic susceptibilities were measured by the modified Evans method. It is found that the electron configuration of the chloroiron corrolates is that of a S = 3/2 Fe(III) center coupled to a corrolate pi radical, where one electron has been removed from the pi system of the corrolate. This pi radical is antiferromagnetically coupled to the unpaired electrons of the iron to yield an overall S = 1 complex, as evidenced by the very large positive shifts of the meso-H resonances (183 and 172 ppm). That this antiferromagnetic coupling is very strong is supported by the near-Curie behavior of the 1H chemical shifts. For the chloroiron corrolates in the presence of imidazole, imidazole-d4, and N-methylimidazole at temperatures of -50 degrees C and below, the mono- and bisligand complexes are formed. The NMR spectra can be assigned on the basis of chemical exchange between the chloroiron(III) parent complex and the bisligand complex at -30 degrees C, and between the bisligand complex and the monoligand complex at -50 degrees C. The bisimidazole complexes show pyrrole CH2 and CH3 resonances characteristic of low-spin Fe(III) centers (S = 1/2), but with strongly upfield-shifted meso-H resonances (delta values of -95 and -82.5 ppm for the octamethyl complex and -188 and -161 ppm for the dimethylhexaethyl complex at 203 K) characteristic of the presence of a macrocycle-centered unpaired electron. The magnetic moments of these bisligand complexes are somewhat lower than expected for overall S = 1 systems, and decrease as the temperature is lowered. The lower apparent magnetic moments (2.0-1.8 mu B between -50 and -90 degrees C) are believed to be caused by a combination of weak or no magnetic coupling between the metal and macrocycle electrons and decreasing solubility of the complex as the temperature is lowered. The non-Curie behavior of the 1H chemical shifts observed in the low-temperature (-50 to -90 degrees C) NMR spectra likely arises from a combination of the effects of weak antiferromagnetic coupling of metal and macrocycle spins, a low-lying electronic excited state, and ligand binding/loss equilibria at the highest temperatures studied (-50 degrees C).
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