Control of <i>Saccharomyces cerevisiae</i> pre-tRNA processing by environmental conditions

Foretek, Dominika; Wu, Jingyan; Hopper, Anita K.; Boguta, Magdalena

doi:10.1261/rna.054973.115

Cited by 23 publications

(38 citation statements)

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“…RNA isolation and northern hybridization was done as described previously [39], using 5 µg of RNA separated by electrophoresis on 10% polyacrylamide, 8 M urea gel. The following DIG-labeled oligonucleotides were used for RNA hybridization: tL(CAA) 5'-TATTCCCACAGTTAACTGCGGTC A-3'; tY(GUA) 5'-GAGAGTCGATTTCTTGC-3'; tF(GAA) 5'-GCGCTCTCCCAACTGAGCT-3'; and 5.8S rRNA, 5'-GCGTTGTTCATCGATGC-3'.…”

Section: Northern Analysismentioning

confidence: 99%

Coupling of RNA polymerase III assembly to cell cycle progression in Saccharomyces cerevisiae

et al. 2019

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Assembly of the RNA polymerases in both yeast and humans is proposed to occur in the cytoplasm prior to their nuclear import. Our previous studies identified a cold-sensitive mutation, rpc128-1007, in the yeast gene encoding the second largest Pol III subunit, Rpc128. rpc128-1007 is associated with defective assembly of Pol III complex and, in consequence, decreased level of tRNA synthesis. Here, we show that rpc128-1007 mutant cells remain largely unbudded and larger than wild type cells. Flow cytometry revealed that most rpc128-1007 mutant cells have G1 DNA content, suggesting that this mutation causes pronounced cell cycle delay in the G1 phase. Increased expression of gene encoding Rbs1, the Pol III assembly/import factor, could counteract G1 arrest observed in the rpc128-1007 mutant and restore wild type morphology of mutant cells. Concomitantly, cells lacking Rbs1 show a mild delay in G1 phase exit, indicating that Rbs1 is required for timely cell cycle progression. Using the double rpc128-1007 maf1Δ mutant in which tRNA synthesis is recovered, we confirmed that the Pol III assembly defect associated with rpc128-1007 is a primary cause of cell cycle arrest. Together our results indicate that impairment of Pol III complex assembly is coupled to cell cycle inhibition in the G1 phase. ARTICLE HISTORY

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Section: Northern Analysismentioning

confidence: 99%

Coupling of RNA polymerase III assembly to cell cycle progression in Saccharomyces cerevisiae

et al. 2019

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“…Here we extend this approach by applying it to tRNA-enriched size fragments with the aim to annotate and curate all tRNAs. Since tRNA processing, such as precursor trimming and intron removal, is a fast process (Foretek et al, 2016), we also aimed to enrich specifically for pre-tRNAs in order to identify and annotate the corresponding unique tRNA gene template. Thus, we performed PAR-CLIP on SSB, a conserved and ubiquitous protein involved in 3′ tRNA processing (Bayfield and Maraia, 2009; Bayfield et al, 2010; Stefano, 1984).…”

Section: Introductionmentioning

confidence: 99%

Characterizing Expression and Processing of Precursor and Mature Human tRNAs by Hydro-tRNAseq and PAR-CLIP

et al. 2017

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Summary The participation of transfer RNAs (tRNAs) in fundamental aspects of biology and disease necessitates an accurate, experimentally confirmed annotation of tRNA genes, and curation of tRNA sequences. This has been challenging, because RNA secondary structure, nucleotide modifications and tRNA gene multiplicity, complicate sequencing and mapping efforts. To address these issues, we developed hydro-tRNAseq, a method based on partial alkaline RNA hydrolysis that generates fragments amenable for sequencing. To identify transcribed tRNA genes, we further complemented this approach with Photoactivatable Crosslinking and Immunoprecipitation (PAR-CLIP) of SSB/La, a conserved protein involved in pre-tRNA processing. Our results show that approximately half of all predicted tRNA genes are transcribed in human cells. We also report nucleotide modification sites, their order of introduction, and identify tRNA leaders, trailers and introns. By using complementary sequencing-based methodologies we present a human tRNA atlas, and determine expression levels of mature and processing intermediates of tRNAs in human cells.

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“…Although we are unaware of other animal evidence that La functionally impacts pre-tRNA metabolism, it is accepted that 3= trailer-containing pre-tRNAs are destabilized in yeast with La deleted and stabilized by its overexpression (11,15,(135)(136)(137). Thus, by analogy, it might be expected that the observed decrease in 3= trailer-containing, spliced pre-tRNA Tyr in cKO cortex (46) was due to loss of La binding.…”

Section: Discussionmentioning

confidence: 99%

La Deletion from Mouse Brain Alters Pre-tRNA Metabolism and Accumulation of Pre-5.8S rRNA, with Neuron Death and Reactive Astrocytosis

Blewett

Iben

Gaidamakov

et al. 2017

Molecular and Cellular Biology

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Human La antigen (Sjögren's syndrome antigen B [SSB]) is an abundant multifunctional RNA-binding protein. In the nucleoplasm, La binds to and protects from 3= exonucleases, the ends of precursor tRNAs, and other transcripts synthesized by RNA polymerase III and facilitates their maturation, while a nucleolar isoform has been implicated in rRNA biogenesis by multiple independent lines of evidence. We showed previously that conditional La knockout (La cKO) from mouse cortex neurons results in defective tRNA processing, although the pathway(s) involved in neuronal loss thereafter was unknown. Here, we demonstrate that La is stably associated with a spliced pre-tRNA intermediate. Microscopic evidence of aberrant nuclear accumulation of 5.8S rRNA in La cKO is supported by a 10-fold increase in a pre-5.8S rRNA intermediate. To identify pathways involved in subsequent neurodegeneration and loss of brain mass in the cKO cortex, we employed mRNA sequencing (mRNASeq), immunohistochemistry, and other approaches. This revealed robust enrichment of immune and astrocyte reactivity in La cKO cortex. Immunohistochemistry, including temporal analyses, demonstrated neurodegeneration, followed by astrocyte invasion associated with immune response and decreasing cKO cortex size over time. Thus, deletion of La from postmitotic neurons results in defective pre-tRNA and prerRNA processing and progressive neurodegeneration with loss of cortical brain mass.KEYWORDS La protein, pre-rRNA, tRNA maturation, tRNA splicing L a was described as a component of ribonucleoprotein particles (RNPs) targeted by autoantibodies in patients suffering from systemic lupus erythematosus and Sjögren's syndrome (1) and was later found in all free-living eukaryotes (2). La is an abundant RNA-binding protein that recognizes UUU-3=-OH, which results from transcription termination by RNA polymerase III (RNAP III) (3-5). This conserved activity functions to protect nascent RNAs from 3= exonucleases, including the nuclear exosome Rrp6, and facilitates the ordered processing and maturation of these transcripts, the more abundant of which are the precursor tRNAs (6-12, 15; reviewed in references 13 and 14).In addition to 3=-end protection, La also exhibits RNA chaperone activity, which serves to prevent misfolding of the pre-tRNA sequences with a propensity to form alternate structures (8,14,16,17). The RNA chaperone activity works with the 3= protection activity to assist structurally challenged pre-tRNAs that would otherwise succumb to nuclear surveillance via exosome Rrp6-mediated decay (9,10,15,18,19).La is nonessential in the yeasts Saccharomyces cerevisiae and Schizosaccharomyces pombe (14, 137) but is essential during Drosophila melanogaster and Mus musculus development (20, 21), suggesting that its role in RNAP III transcript maturation is

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Control of Saccharomyces cerevisiae pre-tRNA processing by environmental conditions

Cited by 23 publications

References 50 publications

Coupling of RNA polymerase III assembly to cell cycle progression in Saccharomyces cerevisiae

Coupling of RNA polymerase III assembly to cell cycle progression in Saccharomyces cerevisiae

Characterizing Expression and Processing of Precursor and Mature Human tRNAs by Hydro-tRNAseq and PAR-CLIP

La Deletion from Mouse Brain Alters Pre-tRNA Metabolism and Accumulation of Pre-5.8S rRNA, with Neuron Death and Reactive Astrocytosis

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