Literature DB >> 19180644

Coexpression of alpha 2A-adrenergic and delta-opioid receptors in substance P-containing terminals in rat dorsal horn.

Maureen S Riedl1, Stephen A Schnell, Aaron C Overland, Anne-Julie Chabot-Doré, Anna M Taylor, Alfredo Ribeiro-da-Silva, Robert P Elde, George L Wilcox, Laura S Stone.   

Abstract

Agonists acting at alpha(2)-adrenergic and opioid receptors (alpha(2)ARs and ORs, respectively) inhibit pain transmission in the spinal cord. When coadministered, agonists activating these receptors interact in a synergistic manner. Although the existence of alpha(2)AR/OR synergy has been well characterized, its mechanism remains poorly understood. The formation of heterooligomers has been proposed as a molecular basis for interactions between neuronal G-protein-coupled receptors. The relevance of heterooligomer formation to spinal analgesic synergy requires demonstration of the expression of both receptors within the same neuron as well as the localization of both receptors in the same neuronal compartment. We used immunohistochemistry to investigate the spatial relationship between alpha(2)ARs and ORs in the rat spinal cord to determine whether coexpression could be demonstrated between these receptors. We observed extensive colocalization between alpha(2A)-adrenergic and delta-opioid receptors (DOP) on substance P (SP)-immunoreactive (-ir) varicosities in the superficial dorsal horn of the spinal cord and in peripheral nerve terminals in the skin. alpha(2A)AR- and DOP-ir elements were colocalized in subcellular structures of 0.5 mum or less in diameter in isolated nerve terminals. Furthermore, coincubation of isolated synaptosomes with alpha(2)AR and DOP agonists resulted in a greater-than-additive increase in the inhibition of K(+)-stimulated neuropeptide release. These findings suggest that coexpression of the synergistic receptor pair alpha(2A)AR-DOP on primary afferent nociceptive fibers may represent an anatomical substrate for analgesic synergy, perhaps as a result of protein-protein interactions such as heterooligomerization. (c) 2009 Wiley-Liss, Inc.

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Year:  2009        PMID: 19180644      PMCID: PMC2745955          DOI: 10.1002/cne.21982

Source DB:  PubMed          Journal:  J Comp Neurol        ISSN: 0021-9967            Impact factor:   3.215


  77 in total

1.  Opiate analgesics inhibit substance P release from rat trigeminal nucleus.

Authors:  T M Jessell; L L Iversen
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3.  Regulation of delta-opioid receptor trafficking via mu-opioid receptor stimulation: evidence from mu-opioid receptor knock-out mice.

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4.  Detection of substance P in the central nervous system by a monoclonal antibody.

Authors:  A C Cuello; G Galfre; C Milstein
Journal:  Proc Natl Acad Sci U S A       Date:  1979-07       Impact factor: 11.205

5.  Substance P immunoreactivity in the median eminence of the North American opossum and domestic fowl.

Authors:  R H Ho; L R DePalatis
Journal:  Brain Res       Date:  1980-05-12       Impact factor: 3.252

6.  Hetero-oligomers of alpha2A-adrenergic and mu-opioid receptors do not lead to transactivation of G-proteins or altered endocytosis profiles.

Authors:  Y Q Zhang; L E Limbird
Journal:  Biochem Soc Trans       Date:  2004-11       Impact factor: 5.407

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8.  Actions of noradrenaline on substantia gelatinosa neurones in the rat spinal cord revealed by in vivo patch recording.

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Authors:  Anne Morinville; Catherine M Cahill; Brigitte Kieffer; Brian Collier; Alain Beaudet
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  42 in total

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5.  Protein kinase C mediates the synergistic interaction between agonists acting at alpha2-adrenergic and delta-opioid receptors in spinal cord.

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Review 7.  Disease-specific heteromerization of G-protein-coupled receptors that target drugs of abuse.

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Review 9.  Transmitting pain and itch messages: a contemporary view of the spinal cord circuits that generate gate control.

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10.  Dual allosteric modulation of opioid antinociceptive potency by α2A-adrenoceptors.

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