Structure-Activity Relationships of Rat Neuromedin U for Smooth Muscle Contraction.

Sakura, Naoki; Ohta, Satoru; Uchida, Yoshiki; Kurosawa, Katsuro; Okimura, Keiko; Hashimoto, Tadashi

doi:10.1248/cpb.39.2016

Cited by 32 publications

(20 citation statements)

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“…The same result was obtained for rat neuromedin U-23, 5,14,15) dog neuromedin U-8 bearing pGlu at the N-terminal, 6,16) and [Gly 1 ]-neuromedin U-8, 17) (data not shown). The displacement curves of synthetic N-terminally deleted analogs 5) such as H-Phe-LeuPhe-Arg-Pro-Arg-Asn-NH 2 , H-Leu-Phe-Arg-Pro-Arg-Asn-NH 2 , and H-Phe-Arg-Pro-Arg-Asn-NH 2 showed reduced but considerable cross-reactivity. The C-terminally deleted analogs H-Tyr-Phe-Leu-Phe-Arg-Pro-Arg-OH 6) and [Gly 8 ]-neuromedin U-8 17) showed no activity in displacing the tracer.…”

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confidence: 79%

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Structure-Activity Relationships of Neuromedin U. V. Study on the Stability of Porcine Neuromedin U-8 at the C-Terminal Asparagine Amide under Mild Alkaline and Acidic Conditions

Kawai

Shibata

Kurosawa

et al. 2006

CHEMICAL & PHARMACEUTICAL BULLETIN

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confidence: 79%

“…5) The amino acid analysis data of various synthetic peptides is shown in Table 1, while their FAB-MS analysis data and characteristics are shown in Table 2.…”

mentioning

confidence: 99%

Structure-Activity Relationships of Neuromedin U. V. Study on the Stability of Porcine Neuromedin U-8 at the C-Terminal Asparagine Amide under Mild Alkaline and Acidic Conditions

Kawai

Shibata

Kurosawa

et al. 2006

CHEMICAL & PHARMACEUTICAL BULLETIN

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“…It is known that these structurally highly conserved neuropeptides share a motif of FLFRPRX-amide, suggesting the importance of this sequence in the interaction with its cognate receptors. Specifically, NMU-8 peptides precede with a large flexibility of the 4 amino acids sequence rich in hydrophobic residues, namely Tyr -NH 2 in all species, implying that an amphiphilic structure could be designed [23][24][25][26][27][28][29] . Diphenyl groups are widely present in many drugs on the market targeting GPCR, including adrenergic receptor antagonists, muscarinic receptor antagonists, analgesic agents (opioid receptor agonists), anti-allergic medications (histamine receptor-1 antagonists), and serotonin receptor modulators [34] .…”

Section: Discussionmentioning

confidence: 99%

“…Structural modifications Five groups of analogs to 101586 were designed and synthesized. Compounds 1a-d were designed based on the SAR information relative to porcine NMU-8 [23][24][25][26][27][28][29] . The diphenyl group was introduced to resemble the hydrophobic residues in this peptide, as we believe this group may bind to a hydrophobic site on the hNMU-R, and that an interaction with an anionic site of the receptor might be realized by linking to a cyclized guanidine group with changes in the carbon chain length and ring size.…”

Section: Hts Campaignmentioning

confidence: 99%

Identification of non-peptidic neuromedin U receptor modulators by a robust homogeneous screening assay

Meng

Binkert

et al. 2008

Acta Pharmacologica Sinica

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Aim: To develop a homogeneous binding assay for high-throughput screening (HTS) of hit compounds at human neuromedin U receptor (hNMU-R) 1 and to identify non-peptidic small molecule hNMU-R modulators through functional assessments and structure-activity relationship (SAR) analyses. Methods: Membrane preparations of Chinese hamster ovary cells (CHO-K1) stably expressing hNMU-R1, [ 125 I]hNMU-25, and wheat germ agglutinin-coupled microbeads were used to develop an HTS assay based on scintillation proximity assay (SPA) technology. This method was applied to a large-scale screening campaign against a diverse library of 36 000 synthetic compounds or natural products and subsequent confirmation studies. CHO-K1 cells stably expressing full-length hNMU-R1 or hNMU-R2 and a calcium-sensitive dye were employed to functionally measure intracellular calcium mobilization upon ligand stimulation. Preliminary SAR was determined based on limited structural modifications. Results: The K i value (0.7 nmol/L) of hNMU-25 (the natural ligand) at hNMU-R1 measured by the SPA method was consistent with that reported in the literature, and the Z' factor for this HTS assay was 0.81. A total of 100 hits, showing more than 30% competitive inhibition on [ 125 I]hNMU-25 binding to hNMU-R1, were identified initially, 3 of which were confirmed thereafter to have reasonable hNMU-R1-binding affinities and similar chemical structures. Based on their common molecular skeleton, 203 analogs were synthesized and tested. Among the 16 analogs that retained variable hNMU-R1-binding abilities, 2 elicited calcium influx in both hNMU-R1 and hNMU-R2-expressing cells, but none displayed antagonist activity. Conclusion: The homogeneous hNMU-R1 binding assay is an efficient and robust tool for screening potential hNMU-R modulators. Two non-selective hNMU-R agonists discovered are of low molecular weight nature with novel chemical structures. The preliminary SAR investigation suggests that both the triphenyl and guanidinol groups are crucial to the bioactivities observed.

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“…Neuromedin-U (NmU) was originally isolated from porcine spinal cord by Minamino et al (1985) and was subsequently isolated from a variety of species including rat (NmU-23), human (NmU-25) and frog (NmU-25) (Conlon et al 1988;Domin et al 1989;O'Harte et al 1991). The core active sequence (Phe-LeuPhe-Arg-Pro-Arg-Asn-NH2) lies between residues 2 and 8 and is common to mammalian species Sakura et al 1991).…”

Section: Introductionmentioning

confidence: 99%

Localisation of NMU1R and NMU2R in human and rat central nervous system and effects of neuromedin-U following central administration in rats

et al. 2004

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Rationale: Neuromedin-U (NmU) is an agonist at NMU1R and NMU2R. The brain distribution of NmU and its receptors, in particular NMU2R, suggests widespread central roles for NmU. In agreement, centrally administered NmU affects feeding behaviour, energy expenditure and pituitary output. Further central nervous system (CNS) roles for NmU warrant investigation. Objectives: To investigate the CNS role of NmU by mapping NMU1R and NMU2R mRNA and measuring the behavioural, endocrine, neurochemical and c-fos response to intracerebroventricular (i.c.v.) NmU. Methods: Binding affinity and functional potency of rat NmU was determined at human NMU1R and NMU2R. Expression of NMU1R and NMU2R mRNA in rat and human tissue was determined using semi-quantitative reverse-transcription polymerase chain reaction. In in-vivo studies, NmU was administered i.c.v. to male Sprague-Dawley rats, and changes in grooming, motor activity and pre-pulse inhibition (PPI) were assessed. In further studies, plasma endocrine hormones, v.).Results: NmU bound to NMU1R (K I , 0.11±0.02 nM) and NMU2R (K I , 0.21±0.05 nM) with equal affinity and was equally active at NMU1R (EC 50 , 1.25±0.05 nM) and NMU2R (EC 50 , 1.10±0.20 nM) in a functional assay. NMU2R mRNA expression was found at the highest levels in the CNS regions of both rat and human tissues. NMU1R mRNA expression was restricted to the periphery of both species with the exception of the rat amygdala. NmU caused a marked increase in grooming and motor activity but did not affect PPI. Further, NmU decreased plasma prolactin but did not affect levels of corticosterone, luteinising hormone or thyroid stimulating hormone. NmU elevated levels of 5-HT in the frontal cortex and hypothalamus, with decreased levels of its metabolites in the hippocampus and hypothalamus, but did not affect dopamine function. NmU markedly increased FLI in the nucleus accumbens, frontal cortex and central amygdala.

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Structure-Activity Relationships of Rat Neuromedin U for Smooth Muscle Contraction.

Cited by 32 publications

References 1 publication

Structure-Activity Relationships of Neuromedin U. V. Study on the Stability of Porcine Neuromedin U-8 at the C-Terminal Asparagine Amide under Mild Alkaline and Acidic Conditions

Structure-Activity Relationships of Neuromedin U. V. Study on the Stability of Porcine Neuromedin U-8 at the C-Terminal Asparagine Amide under Mild Alkaline and Acidic Conditions

Identification of non-peptidic neuromedin U receptor modulators by a robust homogeneous screening assay

Localisation of NMU1R and NMU2R in human and rat central nervous system and effects of neuromedin-U following central administration in rats

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