Detection of changes in gene regulatory patterns, elicited by perturbations of the Hsp90 molecular chaperone complex, by visualizing multiple experiments with an animation

Echeverria, Pablo Christian; Forafonov, Fedor; Pandey, Deo Prakash; Mühlebach, Guillaume; Picard, Didier

doi:10.1186/1756-0381-4-15

Cited by 14 publications

(18 citation statements)

References 47 publications

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“…In S. pombe, treatment with geldanamycin increased fbp1 transcription, but the overall expression was 20 % less than the hsp90 (git10) mutation (Alaamery and Hoffman 2008). In addition, there was only about 20 % overlap of targets with altered expression in cells treated with the Hsp90 inhibitor radicicol or containing a deletion in the gene encoding the Hsp90 cochaperone Sba1 (Echeverria et al 2011). It seems likely that many of these effects are due to altered Sgt1 interaction.…”

Section: Hsp90 Interaction With Sgt1 and Cyr1mentioning

confidence: 91%

“…To gain appreciation of how our results compare with transcriptional changes that occur upon general inhibition of Hsp90, we compared the list of genes that displayed altered expression in hsc82-W296A cells with the list of genes affected by Hsp90 inhibition in yeast. A prior study (Echeverria et al 2011) identified 185 genes whose expression changed at least 1.5 log fold either when Hsp90 was inhibited by radicicol and/or when cells contained a deletion in the cochaperone SBA1. A comparison of the two lists showed that only 38, or 20 %, of the genes identified in that study were also affected by hsc82-W296A mutation (Table S3).…”

Section: Hsp90 Interacts With Cyr1 In Vivomentioning

confidence: 99%

“…Sse1, an Hsp70 binding partner required for full activity of Hsp90 client proteins (Liu et al 1999), and the Sch9 kinase, which is known to regulate Hsp90 function , cooperate to regulate PKA activity (Trott et al 2005). More recently, a report demonstrated that treatment with the Hsp90 inhibitor radicicol resulted in the upregulation of 114 genes in yeast, 26 of which contain Msn2/Msn4 binding elements, known as stress-response elements (STREs) (Echeverria et al 2011). Hsp90 regulation of PKA activity also plays a key role in pathogenesis of Candida albicans.…”

Section: Introductionmentioning

confidence: 97%

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Identification of an Hsp90 mutation that selectively disrupts cAMP/PKA signaling in Saccharomyces cerevisiae

2012

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Section: Hsp90 Interaction With Sgt1 and Cyr1mentioning

confidence: 91%

Section: Hsp90 Interacts With Cyr1 In Vivomentioning

confidence: 99%

Section: Introductionmentioning

confidence: 97%

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Identification of an Hsp90 mutation that selectively disrupts cAMP/PKA signaling in Saccharomyces cerevisiae

2012

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“…Interestingly, some previously identified HSP90 client proteins and interactors were found to be than 23 studies in which higher-throughput, unbiased survey approaches have been taken to detect proteins interacting directly or indirectly with HSP90. These studies have commonly involved genetic, chemical genetic and physical interaction screens performed in yeast [8][9][10][11][12][13][14] as well as large-scale analyses, commonly utilizing affinity purification of HSP90, of proteins present in HSP90 complexes. 7,[15][16][17][18][19][20] Only a few efforts have been made previously toward characterizing the global cellular effects of HSP90 inhibition in mammalian cells.…”

Section: Expanding the Hsp90 Proteome Using Silac Technologymentioning

confidence: 99%

The expanding proteome of the molecular chaperone HSP90

2012

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T he molecular chaperone HSP90 maintains the activity and stability of a diverse set of "client" proteins that play key roles in normal and disease biology. Around 20 HSP90 inhibitors that deplete the oncogenic clientele have entered clinical trials for cancer. However, the full extent of the HSP90-dependent proteome, which encompasses not only clients but also proteins modulated by downstream transcriptional responses, is still incompletely characterized and poorly understood. Earlier large-scale efforts to define the HSP90 proteome have been valuable but are incomplete because of limited technical sensitivity. Here, we discuss previous large-scale surveys of proteome perturbations induced by HSP90 inhibitors in light of a significant new study using state-of-the-art stable isotope labeling by amino acids (SILAC) technology combined with more sensitive highresolution mass spectrometry (MS) that extends the catalog of proteomic changes in inhibitor-treated cancer cells. Among wide-ranging changes, major functional responses include downregulation of protein kinase activity and the DNA damage response alongside upregulation of the protein degradation machinery. Despite this improved proteomic coverage, there was surprisingly little overlap with previous studies. This may be due in part to technical issues but is likely also due to the variability of the HSP90 proteome with the inhibitor conditions used, the cancer cell type and the genetic status of client proteins. We suggest future proteomic studies to address these factors, to help distinguish client protein components from indirect transcriptional

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“…Integration of experimental data in protein-protein interaction (PPI) networks to build explorable maps using Cytoscape (http://www.cytoscape.org) has been previously described [29,30]. Briefly, using the human-centred PPI database built by Echeverria et al [31], it was possible to extract a network containing the PPIs between the query proteins and their interactors.…”

Section: Network-based Data Organization and Discoverymentioning

confidence: 99%

An interplay between the p38 MAPK pathway and AUBPs regulates c-fos mRNA stability during mitogenic stimulation

Degese

Tanos

Naipauer

et al. 2015

Biochemical Journal

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Mitogen-activated protein kinase (MAPK) pathways constitute key regulatory elements linking extracellular stimuli to nuclear gene expression. Immediate-early responsive genes (IEGs) of the activator protein 1 (AP-1) family, such as fos, achieve peak expression levels shortly after cells are stimulated with growth factors and sharply decrease thereafter. Several AU-rich binding proteins (AUBPs), including HuR (Hu-antigen R, Elav-like protein 1, ELAVL1) and KSRP (far upstream element-binding protein 2, KHSRP) bind to a fos AU-rich element (ARE) present in the 3'-UTR (untranslated region) of fos mRNA regulating its stability by a still poorly defined mechanism. We show in the present study that, whereas HuR binds and stabilizes transcribed reporter mRNAs bearing the fos 3'-UTR, KSRP counteracts this effect. Furthermore, we found that fos mRNA stability and HuR phosphorylation status are dependent on the activity of p38 MAPK in both epithelial cells and fibroblasts upon proliferative stimulation. Analysing PPI (protein-protein interaction) networks, we performed a thorough query of interacting proteins for p38 MAPKs, HuR and other AUBPs upon growth factor stimulation. This revealed novel HuR interactors including inhibitors of protein phosphatase 2 (PP2A) activity. Over-expression of two of these interactors, pp32 and APRIL (acidic leucine-rich nuclear phosphoprotein 32 family member B, ANP32B) and pharmacological inhibition of PP2A stabilized a fos reporter mRNA. Our results indicate that p38 MAPK regulates fos mRNA decay by affecting the state of phosphorylation of HuR while controlling yet to be fully elucidated PP regulatory networks.

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Detection of changes in gene regulatory patterns, elicited by perturbations of the Hsp90 molecular chaperone complex, by visualizing multiple experiments with an animation

Cited by 14 publications

References 47 publications

Identification of an Hsp90 mutation that selectively disrupts cAMP/PKA signaling in Saccharomyces cerevisiae

Identification of an Hsp90 mutation that selectively disrupts cAMP/PKA signaling in Saccharomyces cerevisiae

The expanding proteome of the molecular chaperone HSP90

An interplay between the p38 MAPK pathway and AUBPs regulates c-fos mRNA stability during mitogenic stimulation

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