Nuclear compartmentalization of TERT mRNA and TUG1 lncRNA is driven by intron retention

Dumbović, Gabrijela; Braunschweig, Ulrich; Langner, Heera K.; Smallegan, Michael J.; Biayna, Josep; Hass, Evan P.; Jastrzębska, Katarzyna; Blencowe, Benjamin J.; Cech, Thomas R.; Caruthers, Marvin H.; Rinn, John L.

doi:10.1038/s41467-021-23221-w

Cited by 33 publications

(30 citation statements)

References 86 publications

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“…MALAT1 is exclusively associated to chromatin (40), whereas DANCR is a well characterized transcript known to be mainly cytoplasmic (41), where it is also translated (26). Consistent with previous results obtained within other cell types (42–44), TUG1 was equally distributed across the nucleoplasm, the chromatin, and cytoplasm within ECs, suggesting that TUG1 might incorporate different functions in ECs.…”

Section: Resultssupporting

confidence: 91%

“…The high levels of TUG1 transcript might serve as a backup for certain stress responses. This was further supported by the findings of Dumbovic et al (44): Intron retention in the TUG1 transcript drives nuclear compartmentalization and the authors hypothesize that this might indeed serve as a system for buffering the TUG1 transcript in particular stress conditions. In addition, TUG1 is involved in diabetic retinopathy in mice (6) and many types of cancer via a nuclear or cytoplasmic function (21, 51, 30, 52, 53).…”

Section: Discussionsupporting

confidence: 66%

supporting

confidence: 79%

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Aging-regulated TUG1 is dispensable for endothelial cell function

Gimbel

Koziarek

Theodorou

et al. 2022

Preprint

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The evolutionary conserved Taurine Upregulated Gene 1 ( TUG1 ) is a ubiquitously expressed gene that is one of the highest expressed genes in human and rodent endothelial cells (ECs). We here show that TUG1 expression decreases significantly in aging mouse carotid artery ECs and human ECs in vitro , indicating a potential role in the aging endothelial vasculature system. We therefore investigated if, and how, TUG1 might function in aging ECs, but despite extensive phenotyping found no alterations in basal EC proliferation, apoptosis, barrier function, migration, mitochondrial function, or monocyte adhesion upon TUG1 silencing in vitro . TUG1 knockdown did slightly and significantly decrease cumulative sprout length upon vascular endothelial growth factor A stimulation in human umbilical vein endothelial cells (HUVECs), though TUG1-silenced HUVECs displayed no transcriptome-wide mRNA expression changes explaining this effect. Further, ectopic expression of the highly conserved and recently discovered 153 amino acid protein translated from certain TUG1 transcript isoforms did not alter angiogenic sprouting in vitro . Our data show that, despite a high expression and strong evolutionary conservation of both the TUG1 locus and the protein sequence it encodes, TUG1 does not seem to play a major role in basic endothelial cell function.

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Section: Resultssupporting

confidence: 91%

Section: Discussionsupporting

confidence: 66%

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Aging-regulated TUG1 is dispensable for endothelial cell function

Gimbel

Koziarek

Theodorou

et al. 2022

Preprint

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“…As described early in the result section, we have re-analyzed and identified more than 350 rG4 in about 200 ncRNAs using our published rG4-seq dataset. In this list ( Supplementary Table S1 ), we also found rG4s in other biologically relevant lncRNAs such as TUG1 (taurine upregulated gene 1) , HCG11 (HLA Complex Group 11) , DGCR5 (DiGeorge Syndrome Critical Region Gene 5) , HOTAIRM1 (HOXA Transcript Antisense RNA, Myeloid-Specific 1), which have been functionally characterized in other studies recently ( 98–105 ). Our view is that this list is likely an underestimation of the rG4s in ncRNAs as the rG4-seq was polyA-enriched ( 5 ), and that many ncRNAs do not have polyA tail or polyA region in their sequences.…”

Section: Discussionmentioning

confidence: 54%

Identification and targeting of G-quadruplex structures in MALAT1 long non-coding RNA

Mou

Liew

Kwok

2021

Nucleic Acids Research

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RNA G-quadruplexes (rG4s) have functional roles in many cellular processes in diverse organisms. While a number of rG4 examples have been reported in coding messenger RNAs (mRNA), so far only limited works have studied rG4s in non-coding RNAs (ncRNAs), especially in long non-coding RNAs (lncRNAs) that are of emerging interest and significance in biology. Herein, we report that MALAT1 lncRNA contains conserved rG4 motifs, forming thermostable rG4 structures with parallel topology. We also show that rG4s in MALAT1 lncRNA can interact with NONO protein with high specificity and affinity in vitro and in nuclear cell lysate, and we provide cellular data to support that NONO protein recognizes MALAT1 lncRNA via rG4 motifs. Notably, we demonstrate that rG4s in MALAT1 lncRNA can be targeted by the rG4-specific small molecule, peptide, and L-aptamer, leading to the dissociation of MALAT1 rG4-NONO protein interaction. Altogether, this study uncovers new and important rG4s in MALAT1 lncRNAs, reveals their specific interactions with NONO protein, offers multiple strategies for targeting MALAT1 and its RNA–protein complex via its rG4 structure and illustrates the prevalence and significance of rG4s in ncRNAs.

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“…We identified 4 such studies [17, 49–51] that validated a total of 9 RIs in our sets of target genes as defined above (5 and 7 in HX1 and iPSC respectively) (Table S3). (The above four plus an additional ten studies [9, 30, 68–75] experimentally validated RIs in an additional 6 and 9 genes that were found in our target gene sets for in HX1 and iPSC respectively, but without evidence of IR in our samples, and 41 and 36 genes, respectively, that did not pass our sample coverage thresholds for inclusion in this study.) The validated intron coordinates (Table S3) were extracted either from the published intron number [17, 49, 50], assuming a count from the gene’s 5’ to 3’ end, or via BLAT queries of the target sequence [51].…”

Section: Methodsmentioning

confidence: 86%

Retained introns in long RNA-seq reads are not reliably detected in sample-matched short reads

David

Maden

Wood

et al. 2022

Preprint

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There is growing interest in retained introns in a variety of disease contexts including cancer and aging. Many software tools have been developed to detect retained introns from short RNA-seq reads, but reliable detection is complicated by overlapping genes and transcripts as well as the presence of unprocessed or partially processed RNAs. We compared introns detected by 5 tools using short RNA-seq reads with introns observed in long RNA-seq reads from the same biological specimens and found: (1) significant disagreement among tools (Fleiss' κ = 0.231) such that 52.4% of all detected intron retentions were not called by more than one tool; (2) that no tool achieved greater than 20% precision or 35% recall under generous conditions; and (3) that retained intron detectability was adversely affected by greater intron length and overlap with annotated exons.

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Nuclear compartmentalization of TERT mRNA and TUG1 lncRNA is driven by intron retention

Cited by 33 publications

References 86 publications

Aging-regulated TUG1 is dispensable for endothelial cell function

Aging-regulated TUG1 is dispensable for endothelial cell function

Identification and targeting of G-quadruplex structures in MALAT1 long non-coding RNA

Retained introns in long RNA-seq reads are not reliably detected in sample-matched short reads

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