Experimental Characterization of Cis-Acting Elements Important for Translation and Transcription in Halophilic Archaea

Brenneis, Mariam; Hering, Oliver; Lange, Christian; Soppa, Jörg

doi:10.1371/journal.pgen.0030229

Cited by 129 publications

(178 citation statements)

References 66 publications

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“…qRT-PCR was performed on total RNA preparations as previously described (Sherwood et al, 2009) using the iQ SYBR Green Supermix and iCycler MyiQ real-time PCR detection system (Bio-Rad) with primers specific for smrs-gfp and ribL10 (ribosomal protein). The ribL10 primers (RibL-RT_f and RibL-RT_r) were as reported elsewhere and served as a normalization control (Brenneis et al, 2007). The smrs-gfp primers were Fw, 59-ACGACTTCTTCAAGAGCG-39, and Rev, 59-CTGCCGTGATGT-ATACGT-39.…”

Section: Methodsmentioning

confidence: 99%

“…Primer pairs were designed to detect the levels of smrs-gfp-specific transcript in total RNA preparations. In addition, the ribL10-specific transcript levels (encoding a ribosomal protein) were determined and served as an unregulated transcript control (Brenneis et al, 2007). The qRT-PCR analysis revealed no dramatic difference in the levels of smrs-gfp-specific transcript among the various strains (i.e.…”

Section: Reduction In Smrs-gfp Levels By Addition Of C-terminal Residmentioning

confidence: 99%

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Hydrophobic carboxy-terminal residues dramatically reduce protein levels in the haloarchaeon Haloferax volcanii

et al. 2010

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Proteolysis is important not only to cell physiology but also to the successful development of biocatalysts. While a wide-variety of signals are known to trigger protein degradation in bacteria and eukaryotes, these mechanisms are poorly understood in archaea, known for their ability to withstand harsh conditions. Here we present a systematic study in which single C-terminal amino acid residues were added to a reporter protein and shown to influence its levels in an archaeal cell. All 20 amino acid residues were examined for their impact on protein levels, using the reporter protein soluble modified red-shifted GFP (smRS-GFP) expressed in the haloarchaeon Haloferax volcanii as a model system. Addition of hydrophobic residues, including Leu, Cys, Met, Phe, Ala, Tyr, Ile and Val, gave the most pronounced reduction in smRS-GFP levels compared with the addition of either neutral or charged hydrophilic residues. In contrast to the altered protein levels, the C-terminal alterations had no influence on smRS-GFP-specific transcript levels, thus revealing that the effect is post-transcriptional.

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Section: Methodsmentioning

confidence: 99%

Section: Reduction In Smrs-gfp Levels By Addition Of C-terminal Residmentioning

confidence: 99%

Hydrophobic carboxy-terminal residues dramatically reduce protein levels in the haloarchaeon Haloferax volcanii

et al. 2010

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“…Long 5Ј UTRs in methanoarchaea were completely unexpected, because previous genomic and experimental analyses had predicted archaeal mRNAs to either be leaderless or possess rather short 5Ј UTRs (27). In addition, a recent systematic screen showed that the majority of haloarchaeal transcripts might be leaderless (28), and a very recent RNA-seq analysis (52) demonstrated that leaderless mRNAs are the rule in S. solfataricus P2. In contrast, the high number of long 5Ј UTRs argue for extensive posttranscriptional regulation at 5Ј UTRs in methanoarchaea (e.g., at the level of transcript stability) by regulatory proteins or RNAs, or through riboswitches.…”

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confidence: 99%

Deep sequencing analysis of the Methanosarcina mazei Gö1 transcriptome in response to nitrogen availability

Jäger

Sharma

Thomsen³

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

187

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Methanosarcina mazei and related mesophilic archaea are the only organisms fermenting acetate, methylamines, and methanol to methane and carbon dioxide, contributing significantly to greenhouse gas production. The biochemistry of these metabolic processes is well studied, and genome sequences are available, yet little is known about the overall transcriptional organization and the noncoding regions representing 25% of the 4.01-Mb genome of M. mazei. We present a genome-wide analysis of transcription start sites (TSS) in M. mazei grown under different nitrogen availabilities. Pyrosequencing-based differential analysis of primary vs. processed 5 ends of transcripts discovered 876 TSS across the M. mazei genome. Unlike in other archaea, in which leaderless mRNAs are prevalent, the majority of the detected mRNAs in M. mazei carry long untranslated 5 regions. Our experimental data predict a total of 208 small RNA (sRNA) candidates, mostly from intergenic regions but also antisense to 5 and 3 regions of mRNAs. In addition, 40 new small mRNAs with ORFs of <30 aa were identified, some of which might have dual functions as mRNA and regulatory sRNA. We confirmed differential expression of several sRNA genes in response to nitrogen availability. Inspection of their promoter regions revealed a unique conserved sequence motif associated with nitrogen-responsive regulation, which might serve as a regulator binding site upstream of the common IIB recognition element. Strikingly, several sRNAs antisense to mRNAs encoding transposases indicate nitrogen-dependent transposition events. This global TSS map in archaea will facilitate a better understanding of transcriptional and posttranscriptional control in the third domain of life.Methanosarcina mazei strain Gö1 is a representative methaneproducing archaeon of ecologic significance because of its role in biogenic methane production in various anaerobic habitats on Earth (1). The genome sequences of M. mazei and its close relatives Methanosarcina acetivorans and Methanosarcina barkeri have recently become available and have revealed an unexpected low proportion of coding region (74.2% in M. acetivorans, 75.15% in M. mazei, and 79.2% in M. barkeri) (2-4). The biochemical basis of methanogenesis has been analyzed in considerable detail (5, 6). In contrast, little is known about global regulatory networks that ensure survival in periods of nutrient starvation or stress in this important group of archaea. More than 50 predicted transcriptional regulators were annotated in the genome of M. mazei. Strikingly, most of them seem to be closely related to bacterial proteins (2), whereas the basic components of the archaeal transcription and translation machineries generally are more similar to those of eukaryotes (7). A recent genetic study (8) discovered the first global transcriptional regulator of M. mazei, the nitrogen regulator NrpR, which was experimentally demonstrated to globally repress transcription of nitrogen fixation and assimilation genes in response to the nitrogen source.Bes...

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“…S2 in the supplemental material). This finding was not surprising, as leaderless transcripts are common to haloarchaea (20,21). An initial analysis was performed in wt cells to assess whether thiamine and/or its metabolic precursors could influence reporter gene expression.…”

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confidence: 83%

ThiN as a Versatile Domain of Transcriptional Repressors and Catalytic Enzymes of Thiamine Biosynthesis

et al. 2017

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Thiamine biosynthesis is commonly regulated by a riboswitch mechanism; however, the enzymatic steps and regulation of this pathway in archaea are poorly understood. Haloferax volcanii, one of the representative archaea, uses a eukaryote-like Thi4 (thiamine thiazole synthase) for the production of the thiazole ring and condenses this ring with a pyrimidine moiety synthesized by an apparent bacterium-like ThiC (2-methyl-4-amino-5-hydroxymethylpyrimidine [HMP] phosphate synthase) branch. Here we found that archaeal Thi4 and ThiC were encoded by leaderless transcripts, ruling out a riboswitch mechanism. Instead, a novel ThiR transcription factor that harbored an N-terminal helix-turn-helix (HTH) DNA binding domain and C-terminal ThiN (TMP synthase) domain was identified. In the presence of thiamine, ThiR was found to repress the expression of thi4 and thiC by a DNA operator sequence that was conserved across archaeal phyla. Despite having a ThiN domain, ThiR was found to be catalytically inactive in compensating for the loss of ThiE (TMP synthase) function. In contrast, bifunctional ThiDN, in which the ThiN domain is fused to an N-terminal ThiD (HMP/HMP phosphate [HMP-P] kinase) domain, was found to be interchangeable for ThiE function and, thus, active in thiamine biosynthesis. A conserved Met residue of an extended ␣-helix near the active-site His of the ThiN domain was found to be important for ThiDN catalytic activity, whereas the corresponding Met residue was absent and the ␣-helix was shorter in ThiR homologs. Thus, we provide new insight into residues that distinguish catalytic from noncatalytic ThiN domains and reveal that thiamine biosynthesis in archaea is regulated by a transcriptional repressor, ThiR, and not by a riboswitch.IMPORTANCE Thiamine pyrophosphate (TPP) is a cofactor needed for the enzymatic activity of many cellular processes, including central metabolism. In archaea, thiamine biosynthesis is an apparent chimera of eukaryote-and bacterium-type pathways that is not well defined at the level of enzymatic steps or regulatory mechanisms. Here we find that ThiN is a versatile domain of transcriptional repressors and catalytic enzymes of thiamine biosynthesis in archaea. Our study provides new insight into residues that distinguish catalytic from noncatalytic ThiN domains and reveals that archaeal thiamine biosynthesis is regulated by a ThiN domain transcriptional repressor, ThiR, and not by a riboswitch.

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Experimental Characterization of Cis-Acting Elements Important for Translation and Transcription in Halophilic Archaea

Cited by 129 publications

References 66 publications

Hydrophobic carboxy-terminal residues dramatically reduce protein levels in the haloarchaeon Haloferax volcanii

Hydrophobic carboxy-terminal residues dramatically reduce protein levels in the haloarchaeon Haloferax volcanii

Deep sequencing analysis of the Methanosarcina mazei Gö1 transcriptome in response to nitrogen availability

ThiN as a Versatile Domain of Transcriptional Repressors and Catalytic Enzymes of Thiamine Biosynthesis

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