Gonadotropin-releasing hormone messenger ribonucleic acid levels are unaltered with changes in the gonadal hormone milieu of the adult male rat

dc.contributor.authorSteiner, Robert A.en_US
dc.contributor.authorWiemann, Jeffrey N.en_US
dc.contributor.authorClifton, Donald K.en_US
dc.date.accessioned2008-10-17T20:41:29Z
dc.date.available2008-10-17T20:41:29Z
dc.date.issued1990-08en_US
dc.description.abstractTesticular function is regulated by the negative feedback effect of sex hormones acting at the brain and pituitary to inhibit the secretion of LH and FSH. An important component of this feedback axis is presumed to involve regulation of secretion and possibly synthesis of GnRH by the brain. We tested the hypothesis that the castration-induced increase in gonadotropin secretion is subserved, at least in part, by increased synthesis of GnRH. Using in situ hybridization and an oligonucleotide probe to pro-GnRH messenger RNA (GnRH mRNA), we compared the level of cellular GnRH mRNA and the relative number of GnRH mRNA-containing neurons between intact and 21-day castrate adult male rats. To derive estimates of the number of GnRH cells and the cellular GnRH mRNA content, coronal sections from each animal were anatomically matched between intact and castrate groups. All identifiable cells within these sections were counted and analyzed with the aid of a computerized image analysis system, by an observer unaware of the animal's experimental group and were assigned an anatomical location for reference. In an initial experiment, we observed no difference in cellular GnRH mRNA signal level between intact (n = 4) and castrate (n = 5) animals (129 +/- 8 vs. 139 +/- 5 grains per cell); however, we did find a statistical difference between the intact and castrated groups in the relative number of GnRH mRNA-containing cells (intact: 212 +/- 15 vs. castrate: 320 +/- 18). To confirm this observation, we repeated the experiment by again comparing the number of GnRH mRNA-positive cells between intact (n = 4) and castrate (n = 4) rats. In this second experiment, we found no difference in the number of identifiable GnRH mRNA-containing cells between intact and castrate animals (272 +/- 14 vs. 274 +/- 36, respectively); this was the case for the total cell count as well as when the data were analyzed by anatomical region. To clarify the conflicting results on cell counts of Exps 1 and 2, we repeated the experiment a third time, again comparing both the number of GnRH mRNA-containing cells and the cellular content of GnRH mRNA. In this experiment, we observed that neither cell number nor content of GnRH mRNA differed between the intact and castrate groups. Again, this was the case for total cell count, as well as when the data were analyzed by anatomical region.(ABSTRACT TRUNCATED AT 400 WORDS)en_US
dc.identifier.citationEndocrinology. 1990 Aug;127(2):523-32en_US
dc.identifier.urihttp://hdl.handle.net/1773/4357
dc.language.isoen_USen_US
dc.publisherEndocrine Societyen_US
dc.subjectmRNAen_US
dc.subjectin situ hybridizationen_US
dc.subjectraten_US
dc.subjectgonadotropin-releasing hormoneen_US
dc.subject.meshRNA Probesen_US
dc.subject.meshOrchiectomyen_US
dc.subject.meshRatsen_US
dc.subject.meshReference Valuesen_US
dc.subject.meshRNA, Messenger, genetics, metabolismen_US
dc.subject.meshBrain, metabolismen_US
dc.subject.meshAnimalsen_US
dc.subject.meshMaleen_US
dc.subject.meshResearch Support, U.S. Gov't, P.H.S.en_US
dc.subject.meshTestosterone, blooden_US
dc.subject.meshGonadorelin, geneticsen_US
dc.subject.meshRats, Inbred Strainsen_US
dc.subject.meshNucleic Acid Hybridizationen_US
dc.subject.meshOligonucleotide Probesen_US
dc.subject.meshNeurons, metabolismen_US
dc.subject.meshHypothalamus, metabolismen_US
dc.subject.meshLuteinizing Hormone, blooden_US
dc.titleGonadotropin-releasing hormone messenger ribonucleic acid levels are unaltered with changes in the gonadal hormone milieu of the adult male raten_US
dc.typeArticleen_US

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