Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Pivot Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Target Concepts:
Gene/Protein
Disease
Symptom
Drug
Enzyme
Compound
Query: EC:3.4.24.11 (
CD10
)
9,792
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Characterization of the distribution of the peptide-degrading enzyme
neutral endopeptidase
-24.11 (E.C. 3.4.24.11;
NEP
; enkephalinase) in the rat brainstem was examined by means of a unique fluorescent histochemical method. Enzyme staining was completely blocked by three potent
NEP
inhibitors (thiorphan, phosphoramidon, and
JHF
-26) at a concentration of 50 nM, supporting the specificity of this method to visualize sites of
NEP
activity selectively. At all levels of the brainstem,
NEP
was localized to cell bodies, cell processes or terminal-like fields and was localized to more than 90 distinct nuclei or subnuclei. In the mesencephalon these included the central gray, cuneiform n., dorsal and lateral tegmental n., inferior colliculus, interpeduncular n., lateral and medial geniculate n., central linear raphe n., mesencephalic n. of the trigeminal nerve, mammillary nuclei, occulomotor n., red n., superior colliculus, ventral n. of the lateral lemniscus, substantia nigra-ventral tegmental area, and the zona incerta. In the pons,
NEP
staining was restricted to fewer regions or nuclei, including the dorsal and ventral cochlear n., facial n., motor trigeminal n., principal sensory trigeminal n., parabrachial nuclei, pontine n., the oral and caudal pontine reticular n., pontine olivary nuclei, several pontine tegmental nuclei, pontine raphe nuclei, and the trapezoid n. In the cerebellum, staining was localized largely to the granule cell layer of the cerebellar cortex. Scattered staining was observed in the molecular cell layer. The medulla contained extensive
NEP
staining localized to nuclei that included the ambiguous n., dorsal motor n. of the vagus, hypoglossal n., inferior olivary n., prepositus hypoglossus n., solitary tract n., nuclei of the spinal tract of the trigeminal n., and the lateral, medial, and superior vestibular nuclei. Nuclei of the medullary reticular formation that were also richly stained for
NEP
included the raphe magnus n., raphe obscurus n., raphe pallidus n., dorsal, lateral, and ventral reticular nuclei of the medulla, and the gigantocellular, lateral paragigantocellular, linear, paramedian and parvicellular reticular nuclei. The widespread distribution of
NEP
in the brainstem suggests the existence of a number of functional systems, including the pathways involved in the mechanisms of pain and analgesia, which are potential targets of
NEP
inhibitors. In most regions, the distribution of
NEP
closely overlapped with that reported for the enkephalins, and showed a more restricted overlap with the reported distribution of substance P.
...
PMID:Fluorescent histochemical localization of neutral endopeptidase-24.11 (enkephalinase) in the rat brainstem. 169 88
A role for
neutral endopeptidase 24.11
(
NEP
) in growth and development is supported by the demonstration that
NEP
hydrolyses and inactivates a number of peptide growth factors including atrial natriuretic peptide, endothelins, bombesin-like peptides, and opioid peptides, including the enkephalins. In the present study, suspensions of cells obtained from the ventral mesencephalon or cortex of rat embryos (ED14) were implanted into the striatum of the adult rat brain. Three to 15 weeks after transplantation the relative distribution of
NEP
-positive cellular elements was visualized histochemically.
NEP
staining in the transplants consistently appeared before
NEP
staining in the surrounding host striatum supporting a relative increase in
NEP
activity in the transplants. The
NEP
staining richly visualized cells of varying size and morphology which lacked the normal organization of the host striatum. The histochemical staining in the transplants and the surrounding host tissue was completely blocked by a 100 nM concentration of the selective
NEP
inhibitors phosphoramidon or
JHF
-26, supporting the exclusive localization of
NEP
by this method.
NEP
localization in the embryonic (ED14) cortex and ventral mesencephalon was also confirmed, suggesting one possible origin for the
NEP
-positive cells visualized in the transplants. Fluorescent double-labeling studies for
NEP
and glial fibrillary acidic protein (GFAP) or transforming growth factor alpha precursor (TGF alpha p) revealed the presence of rich glial labeling within the transplants for both GFAP and TGFap.
NEP
-labeled cells in the transplants were closely associated with glial elements, however, only occasional glial elements in the transplants stained for
NEP
; supporting a non-astrocytic localization for the
NEP
in the transplants. The marked enhancement of
NEP
staining in the transplants may have significance for controlling the rate or pattern of growth of the transplanted cells through inactivation of peptide growth factors produced by, or in response to, the transplants.
...
PMID:Ventral mesencephalic and cortical transplants into the rat striatum display enhanced activity for neutral endopeptidase 24.11 ('enkephalinase'; CALLA). 833 Feb 16
