Identification of a Cytoplasmic Complex That Adds a Cap onto 5′-Monophosphate RNA

Otsuka, Yuichi; Kedersha, Nancy; Schoenberg, Daniel R.

doi:10.1128/mcb.01325-08

Cited by 113 publications

(214 citation statements)

References 35 publications

(55 reference statements)

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“…Thus, these data support our conclusion that CAGE peaks in 39 UTRs are unlikely to represent novel sites of transcription initiation. We conclude that CAGE peaks in 39 UTRs are likely to be associated with transcript degradation products that might be recapped by a recently described cytoplasmic capping complex (Otsuka et al 2009). Thus, the CAGE peaks within 39 UTRs appear to represent 59 ends of cytoplasmic transcript fragments, and not independent promoters.…”

Section: Characterization Of Cage Peaks Within 39 Utrsmentioning

confidence: 53%

Genome-wide analysis of promoter architecture in Drosophila melanogaster

Hoskins

Landolin²,

Brown³

et al. 2010

Genome Res.

224

344

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Core promoters are critical regions for gene regulation in higher eukaryotes. However, the boundaries of promoter regions, the relative rates of initiation at the transcription start sites (TSSs) distributed within them, and the functional significance of promoter architecture remain poorly understood. We produced a high-resolution map of promoters active in the Drosophila melanogaster embryo by integrating data from three independent and complementary methods: 21 million cap analysis of gene expression (CAGE) tags, 1.2 million RNA ligase mediated rapid amplification of cDNA ends (RLM-RACE) reads, and 50,000 cap-trapped expressed sequence tags (ESTs). We defined 12,454 promoters of 8037 genes. Our analysis indicates that, due to non-promoter-associated RNA background signal, previous studies have likely overestimated the number of promoter-associated CAGE clusters by fivefold. We show that TSS distributions form a complex continuum of shapes, and that promoters active in the embryo and adult have highly similar shapes in 95% of cases. This suggests that these distributions are generally determined by static elements such as local DNA sequence and are not modulated by dynamic signals such as histone modifications. Transcription factor binding motifs are differentially enriched as a function of promoter shape, and peaked promoter shape is correlated with both temporal and spatial regulation of gene expression. Our results contribute to the emerging view that core promoters are functionally diverse and control patterning of gene expression in Drosophila and mammals.

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Section: Characterization Of Cage Peaks Within 39 Utrsmentioning

confidence: 53%

Genome-wide analysis of promoter architecture in Drosophila melanogaster

Hoskins

Landolin²,

Brown³

et al. 2010

Genome Res.

224

344

View full text Add to dashboard Cite

show abstract

“…1C as an example). Alternatively, a report identified a component of the cytosolic capping complex that adds a phosphate to monophosphorylated RNA, generating RNA with a 5′-diphosphate (34). Interestingly, RIG-I, a dsRNA-sensing protein, is activated by RNA with either a 5′-triphosphate or a 5′-diphosphate (35).…”

Section: Discussionmentioning

confidence: 99%

Potential role for snoRNAs in PKR activation during metabolic stress

Youssef

Safran

Nakamura

et al. 2015

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

104

103

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Protein kinase RNA-activated (PKR) has long been known to be activated by viral double-stranded RNA (dsRNA) as part of the mammalian immune response. However, in mice PKR is also activated by metabolic stress in the absence of viral infection, and this requires a functional kinase domain, as well as a functional dsRNA-binding domain. The endogenous cellular RNA that potentially leads to PKR activation during metabolic stress is unknown. We investigated this question using mouse embryonic fibroblast cells expressing wild-type PKR (PKR WT ) or PKR with a point mutation in each dsRNA-binding motif (PKR RM ). Using this system, we identified endogenous RNA that interacts with PKR after induction of metabolic stress by palmitic acid (PA) treatment. Specifically, RIP-Seq analyses showed that the majority of enriched RNAs that interacted with WT PKR (≥twofold, false discovery rate ≤ 5%) were small nucleolar RNAs (snoRNAs). Immunoprecipitation of PKR in extracts of UV-cross-linked cells, followed by RT-qPCR, confirmed that snoRNAs were enriched in PKR WT samples after PA treatment, but not in the PKR RM samples. We also demonstrated that a subset of identified snoRNAs bind and activate PKR in vitro; the presence of a 5′-triphosphate enhanced PKR activity compared with the activity with a 5′-monophosphate, for some, but not all, snoRNAs. Finally, we demonstrated PKR activation in cells upon snoRNA transfection, supporting our hypothesis that endogenous snoRNAs can activate PKR. Our results suggest an unprecedented and unexpected model whereby snoRNAs play a role in the activation of PKR under metabolic stress.PKR | snoRNA | metabolic stress | phosphorylation | RNA-binding protein

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“…Demonstration of several Nudix proteins capable of potentially generating RNAs with a 5 ′ monophosphate or diphosphate raises an interesting question regarding the functional consequence of mRNAs with a 5 ′ diphosphate since these would not serve as a substrate for currently known 5 ′ -3 ′ exoribonucleases. However, the recent demonstration that a cytoplasmic 5 ′ -monophosphorylated mRNA can be recapped through a 5 ′ -diphosphorylated intermediate (Otsuka et al 2009;Mukherjee et al 2012) indicates that 5 ′ -diphosphorylated mRNAs may be more efficient substrates for recapping and entry of the mRNA into the translational pool. Whether decapping enzymes that can generate 5 ′ -end diphosphorylated RNAs are involved in facilitating the cytoplasmic recapping pathway remains to be determined.…”

Section: Discussionmentioning

confidence: 99%

Multiple Nudix family proteins possess mRNA decapping activity

Song

Bail

Kiledjian

2013

RNA

120

139

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RNA decapping is an important contributor to gene expression and is a critical determinant of mRNA decay. The recent demonstration that mammalian cells harbor at least two distinct decapping enzymes that preferentially modulate a subset of mRNAs raises the intriguing possibility of whether additional decapping enzymes exist. Because both known decapping proteins, Dcp2 and Nudt16, are members of the Nudix hydrolase family, we set out to determine whether other members of this family of proteins also contain intrinsic RNA decapping activity. Here we demonstrate that six additional mouse Nudix proteins-Nudt2, Nudt3, Nudt12, Nudt15, Nudt17, and Nudt19-have varying degrees of decapping activity in vitro on both monomethylated and unmethylated capped RNAs. The decapping products from Nudt17 and Nudt19 were analogous to Dcp2 and predominantly generated m 7 GDP, while cleavage by Nudt2, Nudt3, Nudt12, and Nudt15 was more pleiotropic and generated both m 7 GMP and m 7 GDP. Interestingly, all six Nudix proteins as well as both Dcp2 and Nudt16 could hydrolyze the cap of an unmethylated capped RNA, indicating that decapping enzymes may be less constrained for the presence of the methyl moiety. Investigation of Saccharomyces cerevisiae Nudix proteins revealed that the yeast homolog of Nudt3, Ddp1p, also possesses decapping activity in vitro. Moreover, the bacterial Nudix pyrophosphohydrolase RppH displayed RNA decapping activity and released m 7 GDP product comparable to Dcp2, indicating that decapping is an evolutionarily conserved activity that preceded mammalian cap formation. These findings demonstrate that multiple Nudix family hydrolases may function in mRNA decapping and mRNA stability.

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Identification of a Cytoplasmic Complex That Adds a Cap onto 5′-Monophosphate RNA

Cited by 113 publications

References 35 publications

Genome-wide analysis of promoter architecture in Drosophila melanogaster

Genome-wide analysis of promoter architecture in Drosophila melanogaster

Potential role for snoRNAs in PKR activation during metabolic stress

Multiple Nudix family proteins possess mRNA decapping activity

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