2017
DOI: 10.1128/mcb.00174-17
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T-Cell Intracellular Antigens and Hu Antigen R Antagonistically Modulate Mitochondrial Activity and Dynamics by Regulating Optic Atrophy 1 Gene Expression

Abstract: Mitochondria undergo frequent morphological changes to control their function. We show here that T-cell intracellular antigens (TIA1b/TIARb) and Hu antigen R (HuR) have antagonistic roles in mitochondrial function by modulating the expression of mitochondrial shaping proteins. Expression of TIA1b/TIARb alters the mitochondrial dynamic network by enhancing fission and clustering, which is accompanied by a decrease in respiration. In contrast, HuR expression promotes fusion and cristae remodeling and increases r… Show more

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Cited by 24 publications
(64 citation statements)
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“…An empty vector (GFP) was used as a negative control, and a vector coexpressing GFP and the RNA-binding protein HuR (human R antigen) was used in some experiments as an additional control ( Fig. 1D) (24,25). We used these cell lines to investigate the three specific regulatory aspects of TIA1 in WDM, namely, regulation of exon 7 splicing in SMN2; the formation, assembly, and/or disassembly of SGs; and effects on mitochondrial dynamics and function (e.g., autophagy, mitophagy, and apoptosis).…”
Section: Resultsmentioning
confidence: 99%
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“…An empty vector (GFP) was used as a negative control, and a vector coexpressing GFP and the RNA-binding protein HuR (human R antigen) was used in some experiments as an additional control ( Fig. 1D) (24,25). We used these cell lines to investigate the three specific regulatory aspects of TIA1 in WDM, namely, regulation of exon 7 splicing in SMN2; the formation, assembly, and/or disassembly of SGs; and effects on mitochondrial dynamics and function (e.g., autophagy, mitophagy, and apoptosis).…”
Section: Resultsmentioning
confidence: 99%
“…GFP (control)-and TIA1-expressing FT293 cells were transiently transfected with SMN1/SMN2 and NF1 minigenes for 24 h. Western blots of GFP-tagged fusion proteins upon tetracycline treatment for 24 h are shown. Analysis of alternative splicing was carried out using RT-PCR assays as described previously (25,44,45). (C to E) Analysis of ectopic SMN1/SMN2 and NF1 alternative splicing in HEK293 (C), SH-SY5Y (D), and C2C12 (E) cells cotransfected with the corresponding minigenes and expression plasmids.…”
Section: Resultsmentioning
confidence: 99%
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“…In addition, TIA1 represses translation of target mRNAs containing adenineand uridine-rich elements (AREs) in the 3 0 UTR (Anderson and Kedersha, 2002;Dixon et al, 2003). At the cellular level, TIA1 regulates lipid storage and membrane dynamics (Heck et al, 2014), recruitment of the protein synthesis machinery to the tubulin cytoskeleton (Li et al, 2014), cell cycle progression (Meyer et al, 2018; Sá nchez-Jimé nez and Izquierdo, 2013), and mitochondrial function (Carrascoso et al, 2017;Tak et al, 2017). Furthermore, these functions of TIA1 are not necessarily intertwined with its role as a component in stress granules during exogenously applied stress.…”
Section: Introductionmentioning
confidence: 99%