Biochemical and functional characterization of high‐affinity urotensin II receptors in rat cortical astrocytes

Castel, Hélène; Diallo, Mickael; Chatenet, David; Leprince, Jérôme; Desrues, Laurence; Schouft, Marie‐Thérèse; Fontaine, Marc; Dubessy, Christophe; Lihrmann, Isabelle; Scalbert, Elisabeth; Malagón, Marı́a M.; Vaudry, Hubert; Tonon, Marie‐Christine; Gandolfo, Pierrick

doi:10.1111/j.1471-4159.2006.04130.x

Cited by 52 publications

(56 citation statements)

References 70 publications

(179 reference statements)

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“…9A). The involvement of PLC in UT signaling has been confirmed in cultured rat cortical astrocytes (Castel et al, 2006;Jarry et al, 2010). IP 3 binds to the IP 3 receptor, a calcium channel on the membrane of the endoplasmic reticulum, resulting in an increase in cytoplasmic calcium levels (Parys and de Smedt, 2012) (Fig.…”

Section: B Signaling Mechanismsmentioning

confidence: 88%

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International Union of Basic and Clinical Pharmacology. XCII. Urotensin II, Urotensin II–Related Peptide, and Their Receptor: From Structure to Function

et al. 2014

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Section: B Signaling Mechanismsmentioning

confidence: 88%

“…Expression of UII mRNA occurs in neurons (Jégou et al, 2006), astrocytes (Castel et al, 2006;Desrues et al, 2012), and endothelial cells .…”

Section: E Distribution Of Urotensin II Receptor In the Central Nervmentioning

confidence: 99%

International Union of Basic and Clinical Pharmacology. XCII. Urotensin II, Urotensin II–Related Peptide, and Their Receptor: From Structure to Function

et al. 2014

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“…Such studies suggest that both ligand and GTP concentration as well as desensitization all play an important role in regulating the ratio of receptor coupling to functionally distinct G-proteins, thereby modulating the precise biological response elicited. In addition, prior studies indicate that cultured rat astrocytes constitutively express both low-affinity and high-affinity GPR14 receptors (Castel et al, 2006). It is plausible that bladder smooth muscle cells also express both low-and high-affinity GPR14 receptors, and that the dose-dependent binding of Urp to these distinct receptor subtypes results in the biphasic regulation of SRF expression in cultured smooth muscle cells.…”

Section: Discussionmentioning

confidence: 99%

Transcriptional profiling of the megabladder mouse: A unique model of bladder dysmorphogenesis

Singh¹,

Robinson²,

Ismail³

et al. 2007

Developmental Dynamics

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Recent studies in our lab identified a mutant mouse model of obstructive nephropathy designated mgb for megabladder. Homozygotic mgb mice (mgb؊/؊) develop lower urinary tract obstruction in utero due to a lack of bladder smooth muscle differentiation. This defect is the result of a random transgene insertion/translocation into chromosomes 11 and 16. Transcriptional profiling identified a significantly over-expressed cluster of gene products located on the translocated fragment of chromosome 16 including urotensin II-related peptide (Urp), which was shown to be preferentially over-expressed in developing mgb؊/؊ bladders. Pathway analysis of mgb microarray data indicated dysregulation of at least 60 gene products associated with smooth muscle development. In conclusion, the results of this study indicate that the molecular pathways controlling normal smooth muscle development are severely altered in mgb؊/؊ bladders, and provide the first evidence that Urp may play a critical role in bladder smooth muscle development. Developmental Dynamics 237:170 -186, 2008.

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“…For example, the effect of U-II was abolished by thapsigargin, indicating the participation of endoplasmic reticulum Ca 2+ pools in rhabdomyosarcoma cell line [27] as well as in frog motor nerve terminals [12]. In rat, rabbit and cat blood vessels [2,32,55,56,61] and in rat cultured astrocytes [16], the effect of U-II was inhibited by the phospholipase C inhibitor U-73122, indicating the involvement of phospholipase-C/IP 3 pathways. In contrast, U-II elevated [Ca 2+ ] i largely by facilitating Ca 2+ entry through plasmalemmal Ca 2+ channels in rat spinal motoneurons [30].…”

Section: Discussionmentioning

confidence: 98%

State-dependent calcium mobilization by urotensin-II in cultured human endothelial cells

et al. 2008

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Human endothelial cells express urotensin II (U-II) as well as its receptor GPR14. Using microfluorimetric techniques, the effect of human U-II on cytosolic Ca 2+ concentrations [Ca 2+] i in cultured human aortic endothelial cells (HAEC) loaded with Fura-2 was evaluated in static or flow conditions. Under the static state, U-II (100 nM) abolished spontaneous Ca 2+ oscillations, which occurred in a population of cultured HAEC. Similarly, U-II reduced thrombin-, but not ATP-induced calcium responses, suggesting that the peptide does not alter the G q/11 /IP 3 pathway; rather, it modifies the coupling between protease activated receptors and G q/11 /IP 3 . Under the flow condition, U-II (1, 10 and 100 nM) produced a dose-dependent increase in [Ca 2+ ] i , which was subjected to desensitization. The result demonstrates a state-dependent effect of U-II in cultured HAEC, which may explain the variable responses to U-II under different experimental conditions.

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Biochemical and functional characterization of high‐affinity urotensin II receptors in rat cortical astrocytes

Cited by 52 publications

References 70 publications

International Union of Basic and Clinical Pharmacology. XCII. Urotensin II, Urotensin II–Related Peptide, and Their Receptor: From Structure to Function

International Union of Basic and Clinical Pharmacology. XCII. Urotensin II, Urotensin II–Related Peptide, and Their Receptor: From Structure to Function

Transcriptional profiling of the megabladder mouse: A unique model of bladder dysmorphogenesis

State-dependent calcium mobilization by urotensin-II in cultured human endothelial cells

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