Reconstitution and analyses of RNA interactions with eukaryotic translation initiation factors and ribosomal preinitiation complexes

Liu, Xiaozhuo; Schuessler, Peter J.; Sahoo, Ansuman; Walker, Sarah E.

doi:10.1016/j.ymeth.2019.03.024

Cited by 11 publications

(25 citation statements)

References 22 publications

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“…40S subunit (and 80S/polysome) containing fractions were verified from the same samples by blotting yeast ribosomal small subunit protein Rps2 (Aviva ARP63572_P050, 1:2000 dilution.) Rabbit antibodies to purified recombinant yeast eIF4A (1:20,000 dilution) and eIF4G1 (1:1000 dilution), generated by Invitrogen/Pierce custom antibody services and verified against the recombinant proteins, were used to determine the position of those proteins within gradients ( Liu et al, 2019 ). Each experiment was repeated three or more times from biological replicates.…”

Section: Methodsmentioning

confidence: 99%

Deletion of the N-Terminal Domain of Yeast Eukaryotic Initiation Factor 4B Reprograms Translation and Reduces Growth in Urea

Liu

Moshiri

et al. 2022

Front. Mol. Biosci.

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The yeast eukaryotic initiation factor 4B binds the 40S subunit in translation preinitiation complexes (PICs), promoting mRNA recruitment. Recent evidence indicates yeast mRNAs have variable dependence on eIF4B under optimal growth conditions. Given the ability of eIF4B to promote translation as a function of nutrient conditions in mammalian cells, we wondered if eIF4B activities in translation could alter phenotypes in yeast through differential mRNA selection for translation. Here we compared the effects of disrupting yeast eIF4B RNA- and 40S-binding motifs under ∼1400 growth conditions. The RNA-Recognition Motif (RRM) was dispensable for stress responses, but the 40S-binding N-terminal Domain (NTD) promoted growth in response to stressors requiring robust cellular integrity. In particular, the NTD conferred a strong growth advantage in the presence of urea, which may be important for pathogenesis of related fungal species. Ribosome profiling indicated that similar to complete eIF4B deletion, deletion of the NTD dramatically reduced translation, particularly of those mRNAs with long and highly structured 5-prime untranslated regions. This behavior was observed both with and without urea exposure, but the specific mRNA pool associated with ribosomes in response to urea differed. Deletion of the NTD led to relative increases in ribosome association of shorter transcripts with higher dependence on eIF4G, as was noted previously for eIF4B deletion. Gene ontology analysis indicated that proteins encoded by eIF4B NTD-dependent transcripts were associated with the cellular membrane system and the cell wall, while NTD-independent transcripts encoded proteins associated with cytoplasmic proteins and protein synthesis. This analysis highlighted the difference in structure content of mRNAs encoding membrane versus cytoplasmic housekeeping proteins and the variable reliance of specific gene ontology classes on various initiation factors promoting otherwise similar functions. Together our analyses suggest that deletion of the eIF4B NTD prevents cellular stress responses by affecting the capacity to translate a diverse mRNA pool.

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Section: Methodsmentioning

confidence: 99%

Deletion of the N-Terminal Domain of Yeast Eukaryotic Initiation Factor 4B Reprograms Translation and Reduces Growth in Urea

Liu

Moshiri

et al. 2022

Front. Mol. Biosci.

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“…Polyclonal anti-eIF4A antibody was further purified from 40 ml of serum by running over a 5 ml Protein A column (Acrobiosystems Inc., MA-0422-C5) for immunoprecipitation experiments. Custom antibodies were verified against recombinant protein (23) and optimized for linear behavior using lysates from BY4741 yeast. Antibodies were used at the following concentrations for western blotting: rabbit anti-eIF4A (1:20000 dilution, custom), rabbit anti-eIF4G (1:1000, custom), and mouse anti-HA (1:5000, Invitrogen, 26183).…”

Section: Methodsmentioning

confidence: 99%

Section: Antibodiesmentioning

confidence: 99%

Dynamic Phosphorylation Regulates Eukaryotic Translation Initiation Factor 4A Activity During the Cell Cycle

Sahoo

Zollo

Shen

et al. 2022

Preprint

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The eukaryotic translation initiation factor 4A (eIF4A) resolves mRNA structures to support protein synthesis, yet little is known about its regulation. Here we analyzed eIF4A phosphorylation during alternate stages of the cell cycle, and found three residues near the DEAD box motif (T73, T146, and S177) underwent substantial phosphorylation changes. Phosphomimetic mutations T73D and T146D led to G2/M phase arrest, and abolished eIF4A interaction with RNA, suggesting eIF4A activity is needed for completion of cell division. In addition to these repressive events, we found that S177, a site immediately adjacent to the DEAD-box, showed diametrically opposed phosphorylation, with only phosphorylated S177 present during G1/S arrest and dephosphorylated S177 peptides during G2/M arrest. Phosphomimetic S177D eIF4A increased polysome levels and enhanced normally reduced eIF4A-eIF4G-interaction during G2/M, while phosphodeficient S177A decreased polysome levels and reduced growth, suggesting phosphorylation of S177 enhances eIF4A-mediated translation during G1/S. Together these results suggest that dynamic phosphorylation of eIF4A S177 serves to stimulate translation during G1/S, while inhibitory phosphorylation of additional sites holds the potential to rapidly transition eIF4A to an inactive state and turn off translation. These results also suggest an important role for eIF4A in coupling translation to cell cycle stages.

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“…The plasmid containing recombinant full-length eIF4G1 was a gift from Sarah Walker (also available on Addgene as plasmid #122248). This full-length eIF4G1 construct with a C-terminal chitin binding domain fusion was purified according to a published procedure (Liu et al, 2019), with the following modifications: the cells were lysed using a sonicator, and the final protein after elution was stored in 250 mM KCl instead of 250 mM KOAc, skipping the dialysis after the anionexchange chromatography step in the procedure, and DTT for storage was substituted with 2.5 mM TCEP. Briefly, E. coli cells expressing full-length eIF4G1 were thawed, and lysed using a sonicator after resuspending in Intein Lysis Buffer (50 mM HEPES-KOH, pH 7.4, 500 mM KCl, 1 mM EDTA).…”

Section: Protein Purification and Labelingmentioning

confidence: 99%

mRNA- and factor-driven dynamic variability controls eIF4F-cap recognition for translation initiation

Çetin

2021

Preprint

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mRNA 5′ cap recognition by eIF4F is a key step in eukaryotic translational control. While different mRNAs respond differently to eIF4F–directed regulation, the molecular basis for this variability remains unclear. We developed single-molecule fluorescence assays to directly observe eIF4F–mRNA interactions. We uncovered a complex interplay of mRNA features with factor activities that differentiates cap recognition between mRNAs. eIF4E–cap association rates are anticorrelated with mRNA length. eIF4A leverages ATP binding to differentially accelerate eIF4E–mRNA association; the extent of this acceleration correlates with translation efficiency in vivo. eIF4G lengthens eIF4E–cap binding to persist on the initiation timescale. The full eIF4F complex discriminates between mRNAs in an ATP-dependent manner. After eIF4F–mRNA binding, eIF4E is ejected from the cap by eIF4A ATP hydrolysis. Our results suggest features throughout mRNA coordinate in controlling cap recognition at the 5ʹ end, and suggest a model for how eIF4F–mRNA dynamics establish mRNA sensitivity to translational control processes.

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Reconstitution and analyses of RNA interactions with eukaryotic translation initiation factors and ribosomal preinitiation complexes

Cited by 11 publications

References 22 publications

Deletion of the N-Terminal Domain of Yeast Eukaryotic Initiation Factor 4B Reprograms Translation and Reduces Growth in Urea

Deletion of the N-Terminal Domain of Yeast Eukaryotic Initiation Factor 4B Reprograms Translation and Reduces Growth in Urea

Dynamic Phosphorylation Regulates Eukaryotic Translation Initiation Factor 4A Activity During the Cell Cycle

mRNA- and factor-driven dynamic variability controls eIF4F-cap recognition for translation initiation

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