Posttranscriptional Regulation of <i>PARG</i> mRNA by HuR Facilitates DNA Repair and Resistance to PARP Inhibitors

Chand, Saswati N.; Zarei, Mahsa; Schiewer, Matthew J.; Kamath, Akshay R.; Romeo, Carmella; Lal, Shruti; Cozzitorto, Joseph A.; Nevler, Avinoam; Scolaro, Laura; Londin, Eric; Jiang, Wei; Meisner‐Kober, Nicole; Pishvaian, Michael J.; Knudsen, Karen E.; Yeo, Charles J.; Pascal, John M.; Winter, Jordan M.; Brody, Jonathan R.

doi:10.1158/0008-5472.can-16-2704

Cited by 60 publications

(68 citation statements)

References 64 publications

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“…In the process, HuR is thought to bind to target mRNA and then form an HuR‐mRNA complex in the nucleus, which is then exported to the cytoplasm to protect the bound mRNA from degradation. There is mounting experimental evidence suggesting that there is an increase in cytoplasmic HuR after stimulation, which is considered a crucial step in the increased stability of many HuR‐bound mRNAs . In accordance with this model, our immunofluorescent staining findings indicate that IL‐4 can also regulate HuR for nuclear shuttle.…”

Section: Discussionsupporting

confidence: 87%

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Interleukin‐4‒induced posttranscriptional gene regulation of CCL26 by the RNA‐binding protein HuR in primary human nasal polyp‒derived epithelial cells

Tian

et al. 2018

Int Forum Allergy Rhinol

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Background: Much a ention on the pathophysiology of nasal polyp (NP) has focused on eosinophils. Interleukin (IL)-4 and eotaxin-3 (C-C motif chemokine ligand 26, or CCL26) levels have been reported to be increased in eosinophilic nasal polyps. The aim of this study was to characterize CCL26 pos ranscriptional regulation by the RNAbinding protein HuR in primary human nasal polyp-derived epithelial cells (hNPDECs) challenged with IL-4. Methods:A prospective, observational study was conducted. Nasal polyp tissues were obtained from eosinophilic (n = 12) and non-eosinophilic (n = 10) NP patients, and inferior turbinate (IT) tissues were taken from control subjects (n = 9) and cultured into hNPDECs. Expression of HuR and CCL26 were measured by immunohistochemistry, Western blot analysis, enzyme-linked immunoassay, and real-time polymerase chain reaction (PCR). The nucleocytoplasmic shu ling of HuR in hNPDECs was detected by immunofluorescence. Pos ranscriptional regulation of CCL26 by HuR was tested by ribonucleoprotein immunoprecipitation assay (RIP) and dual-luciferase reporter assay. CCL26 mRNA stabilization was measured by quatititative PCR a er treatment with actinomycin D. Student's t test and one-way analysis of variance were used.Results: Immunohistochemical data show that both HuR and CCL26 were highly expressed in NP tissues, especially eosinophilic NP tissues (p < 0.05). IL-4 stimulation increased CCL26 mRNA stability, and overexpression and knockdown of HuR affected CCL26 expression. Immunofluorescence data indicate that IL-4 altered the subcellular distribution of HuR. The RIP and dual-luciferase reporter assay results supply strong evidence for HuR binding to CCL26. Conclusion:Our results provide strong support for the hypothesis that IL-4-induced expression of CCL26 in hN-PDECs relies partly on CCL26 mRNA stabilization mediated by the interaction of HuR with CCL26 3'UTR. C 2018 ARS-AAOA, LLC.

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Section: Discussionsupporting

confidence: 87%

“…The posttranscriptional events associated with adenylate‐ and uridylate‐rich elements (AREs)‒containing gene are recognized as important control points in gene regulation . The mechanisms of mRNA decay regulation are closely associated with specific target regions, including AREs in the 3' untranslated regions (3'UTRs) of mRNA .…”

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confidence: 99%

Interleukin‐4‒induced posttranscriptional gene regulation of CCL26 by the RNA‐binding protein HuR in primary human nasal polyp‒derived epithelial cells

Tian

et al. 2018

Int Forum Allergy Rhinol

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“…Furthermore, poly(ADP‐ribose) glycohydrolase (PARG), which hydrolyzes PAR moieties, harbors patient‐derived alterations of unknown relevance, which may impact PARP‐1 activation status by differentially regulating PAR levels. It has recently been reported that PARG impacts the response to PARPi in models of pancreatic cancer (Chand et al , ). Irrespective of the mechanism(s) by which PARP‐1 is hyperactivated in advanced PCa, studies described herein yield novel insights into the downstream functions of elevated PARP‐1 activity.…”

Section: Discussionmentioning

confidence: 99%

PARP‐1 regulates DNA repair factor availability

et al. 2018

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PARP‐1 holds major functions on chromatin, DNA damage repair and transcriptional regulation, both of which are relevant in the context of cancer. Here, unbiased transcriptional profiling revealed the downstream transcriptional profile of PARP‐1 enzymatic activity. Further investigation of the PARP‐1‐regulated transcriptome and secondary strategies for assessing PARP‐1 activity in patient tissues revealed that PARP‐1 activity was unexpectedly enriched as a function of disease progression and was associated with poor outcome independent of DNA double‐strand breaks, suggesting that enhanced PARP‐1 activity may promote aggressive phenotypes. Mechanistic investigation revealed that active PARP‐1 served to enhance E2F1 transcription factor activity, and specifically promoted E2F1‐mediated induction of DNA repair factors involved in homologous recombination (HR). Conversely, PARP‐1 inhibition reduced HR factor availability and thus acted to induce or enhance “BRCA‐ness”. These observations bring new understanding of PARP‐1 function in cancer and have significant ramifications on predicting PARP‐1 inhibitor function in the clinical setting.

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“…Transcriptome wide analysis of samples from cells exposed to IR radiation revealed a decrease in HuR binding to its target mRNAs due to activated CHK2‐mediated phosphorylation (Masuda et al, ). Upon genotoxic stress, HuR can be PARylated by poly(ADP‐ribose) polymerase 1 (PARP1) facilitating its cytoplasmic translocation and regulation of its binding to target mRNAs (Chand et al, ; Gagné et al, ; Y. Ke et al, ). dePARylation of HuR facilitates its release from target mRNAs and its shuttling back into the nucleus.…”

Section: Deadenylation: Rbps and Micrornasmentioning

confidence: 99%

Connections between 3′ end processing and DNA damage response: Ten years later

Murphy

Kleiman

2019

WIREs RNA

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Ten years ago we reviewed how the cellular DNA damage response (DDR) is controlled by changes in the functional and structural properties of nuclear proteins, resulting in a timely coordinated control of gene expression that allows DNA repair. Expression of genes that play a role in DDR is regulated not only at transcriptional level during mRNA biosynthesis but also by changing steady‐state levels due to turnover of the transcripts. The 3′ end processing machinery, which is important in the regulation of mRNA stability, is involved in these gene‐specific responses to DNA damage. Here, we review the latest mechanistic connections described between 3′ end processing and DDR, with a special emphasis on alternative polyadenylation, microRNA and RNA binding proteins‐mediated deadenylation, and discuss the implications of deregulation of these steps in DDR and human disease. This article is categorized under: RNA Processing > 3′ End Processing RNA‐Based Catalysis > Miscellaneous RNA‐Catalyzed Reactions RNA in Disease and Development > RNA in Disease

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Posttranscriptional Regulation of PARG mRNA by HuR Facilitates DNA Repair and Resistance to PARP Inhibitors

Cited by 60 publications

References 64 publications

Interleukin‐4‒induced posttranscriptional gene regulation of CCL26 by the RNA‐binding protein HuR in primary human nasal polyp‒derived epithelial cells

Interleukin‐4‒induced posttranscriptional gene regulation of CCL26 by the RNA‐binding protein HuR in primary human nasal polyp‒derived epithelial cells

PARP‐1 regulates DNA repair factor availability

Connections between 3′ end processing and DNA damage response: Ten years later

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