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Maximal Stimulation (maximal + stimulation)
Selected AbstractsThe Secretory Response of the Rat Colon to the Flavonol Quercetin is Dependent on Ca2+ -CalmodulinEXPERIMENTAL PHYSIOLOGY, Issue 3 2000R. Cermak The dietary flavonol quercetin induces chloride secretion in rat intestine. To clarify the underlying mechanisms, experiments were performed in Ussing chambers with tissue from rat proximal and distal colon. Quercetin induced an increase in short-circuit current (Isc), which was largely independent of submucosal neurons, as it was not affected by the neurotoxin tetrodotoxin. The effect of quercetin was blocked by the calmodulin antagonists trifluoperazine and ophiobolin A and was diminished by a blocker of Ca2+ release from intracellular stores (TMB-8), whereas the muscarinic receptor antagonist atropine was ineffective. The quercetin-induced Isc was abolished in Ca2+ -free solution. The flavonol was able to further increase Isc after maximal stimulation of the cAMP pathway by forskolin. The Isc increase by the flavonol was differently affected by two analogous phosphodiesterase inhibitors. Whereas 3-isobutyl-1-methylxanthine (IBMX) antagonized the effect of quercetin, 8-methoxymethyl-IBMX had no effect. Both phosphodiesterase inhibitors similarly influenced the Isc increase induced by forskolin. These results indicate that the chloride secretion induced by quercetin in rat colon depends on Ca2+ and calmodulin. The cAMP pathway and inhibition of phosphodiesterase appear not to be responsible for the secretory activity of the flavonol. [source] Cadmium-induced hormetic effect in differentiated Caco-2 cells: ERK and p38 activation without cell proliferation stimulationJOURNAL OF CELLULAR PHYSIOLOGY, Issue 1 2010Marc Mantha Cadmium (Cd) is a toxic metal that enters the food chain. Following oral ingestion, the intestinal epithelium may in part protect against Cd toxicity but is also a target tissue. Using human enterocytic-like Caco-2 cells, we have previously shown differences in sensitivity to Cd according to the differentiation status. The present study focuses on Cd effects on differentiated cells. Concentration and time-dependent increases in MTT (3-[4,5-dimethyl-2-thiazol-2-yl]-2,5-diphenyltetrazolium bromide assay) activity were observed in post-confluent cultures exclusively, with a twofold maximal stimulation in 21-day-old cells exposed to 10,µM Cd for 24,h. No concomitant increase in [methyl- 3H] thymidine incorporation was noted and Cd did not modify cell distribution in the cell-cycle phases. However, Cd-induced increase in MTT activity was inhibited by cycloheximine as well as by inhibitors of ERK1/2 and p38, but not by that of JNK. Consistently, Cd increased the levels of ERK1/2 and p38 phosphorylation. Inhibition of Ras-GTP or PI3K enhanced the stimulatory effect of Cd, whereas mTOR inhibition had no effect. Inhibition of G protein-phospholipase and PKC decreased MTT stimulation. These results show a hormesis-like stimulation of Cd on MTT activity in differentiated intestinal cells exclusively. This effect is not related to cell proliferation but more likely to increased protein synthesis which involves ERK1/2 and p38 cascades and possibly PLC-, signaling pathways. Because growth-related differentiation of intestinal cells is linked to the selective and sequential activation of MAPKs, the impacts that these Cd-induced perturbations in signaling pathways may have on intestinal functions clearly deserve to be investigated. J. Cell. Physiol. 224:250,261, 2010 © 2010 Wiley-Liss, Inc. [source] Induction of collagenase-2 (matrix metalloproteinase-8) gene expression by interleukin-1, in human gingival fibroblastsJOURNAL OF PERIODONTAL RESEARCH, Issue 3 2001M. Abe Collagenase-2 (matrix metalloproteinase-8 or MMP-8) is synthesized mainly by polymorphonuclear neutrophils and plays a crucial role in inflammatory periodontal tissue destruction. We tested the effect of interleukin(IL)-1,, a proinflammatory cytokine, on collagenase-2 gene expression in cultured human gingival fibroblasts and also compared this effect with IL-1,-induced changes in collagenase-1 and -3 gene expression. By a combination of reverse transcription-polymerase chain reaction and Southern analysis, IL-1, was found to dose-dependently induce gene expression for collagenase-1, -2, and -3 in gingival fibroblasts. Although collagenase-2 mRNA was the least abundant among the three collagenase mRNAs tested in the cultured fibroblast system, addition of 1 ng/ml IL-1, significantly increased collagenase-2 gene transcription within 6 h, and maximal stimulation was maintained for 12 to 48 h. Significant mRNA induction was observed with as little as 0.1 ng/ml IL-1,. IL-1, was also found to increase the stability of collagenase-2 mRNAs after transcription arrest was induced by an RNA polymerase inhibitor. Stimulation of collagenase-2 mRNA expression by IL-1, was prevented by pretreatment with cycloheximide, an inhibitor of protein synthesis. These results indicate that IL-1, increased mRNA expression for collagenases including collagenase-2 in gingival fibroblasts. The findings also suggest that enhancement of collagenase-2 mRNA expression by IL-1, involves both protein synthesis and suppression of mRNA degradation. [source] A Qualitative and Quantitative Approach to Determine the Optimum Combination of Feeding Stimulants for Striped Bass Morone saxatilis Using an Agar Gel CarrierJOURNAL OF THE WORLD AQUACULTURE SOCIETY, Issue 1 2002Elias Papatryphon A series of experiments was conducted to determine the optimum combination of previously identified feeding stimulants (FS), namely L-alanine (Ala), L-serine (Ser), inosine-5,-monophosphate (IMP), and betaine (Bet), for striped bass Morone saxatilis. Three experiments were conducted to determine the optimum combination of FS using an agar gel matrix as a carrier. In the first experiment a 24 factorial experiment was conducted to test all possible combinations of the four FS at two levels, 0 and 0.1 M. Significant interactions between the FS were found, suggesting the complexity of gustatory stimulation and palatability. In the second experiment a 4 × 6 factorial design was employed to test each FS alone and at concentrations ranging from 0 to 8% in order to determine the minimum level at which maximal stimulation is achieved. The results suggest that there is no significant improvement in feed intake beyond the 1 % level of supplementation for all the FS. In addition, Ala produced a significantly greater response compared to all other FS. In the last experiment, a modified single factor method was used to estimate the optimum levels for each FS in a mixture. The range of the concentrations tested was 0,1% of the agar gel for each FS. Combining all four compounds yielded maximal stimulation. The levels of each compound in the final optimum combination of FS were: Ala, 0.4; Ser, 0.6; Bet, 0.4; and IMP, 0.3% of the agar gel. [source] HongrES1, a cauda epididymis-specific protein, is involved in capacitation of guinea pig sperm,MOLECULAR REPRODUCTION & DEVELOPMENT, Issue 10 2009Ya Ni Capacitation requires removal of proteins secreted by the cauda epididymis. Previously, we isolated and cloned the HongrES1 gene from rat cauda epididymis and found that it was exclusively expressed there. Here we report that HongrES1 mRNA is also expressed in the guinea pig cauda epididymis using Northern blot analysis, and the molecular weight of its cognate protein is approximately 48,kDa by Western blot analysis. Therefore, we investigated whether HongrES1 was involved in regulation of sperm capacitation in guinea pig. The results show that HongrES1 antisera (HA) significantly enhances sperm capacitation with maximal stimulation at a dilution of 1:500. Capacitation was reversed when capacitated spermatozoa were re-exposed to HongrES1 protein (HP, 0.25,µg/ml). In other words, HP acted as a decapacitation factor. HA accelerated the onset of capacitation and promoted a sperm hyperactivated motility response. Sperm capacitation was accelerated by HA stimulation of extracellular calcium influx while HP prevented extracellular calcium from influxing. Indirect immunofluorescence staining finds HP localized over the acrosomal anterior region of the sperm head, which exfoliates gradually during capacitation incubation, and completely disappeared after the acrosome reaction. Thus, HongrES1 expressed by the cauda epididymis is a novel molecule that regulates the physiology of guinea pig sperm prior to fertilization. Mol. Reprod. Dev. 76: 984,993, 2009. © 2009 Wiley-Liss, Inc. [source] Oleamide is a selective endogenous agonist of rat and human CB1 cannabinoid receptorsBRITISH JOURNAL OF PHARMACOLOGY, Issue 2 2004James D Leggett The ability of the endogenous fatty acid amide, cis -oleamide (ODA), to bind to and activate cannabinoid CB1 and CB2 receptors was investigated. ODA competitively inhibited binding of the nonselective cannabinoid agonist [3H]CP55,940 and the selective CB1 antagonist [3H]SR141716A to rat whole-brain membranes with Ki values of 1.14 ,M (0.52,2.53 ,M, Hill slope=0.80, n=6) and 2.63 ,M (0.62,11.20 ,M, Hill slope=0.92, n=4), respectively. AEA inhibited [3H]CP55,940 binding in rat whole-brain membranes with a Ki of 428 nM (346,510 nM, Hill slope=,1.33, n=3). ODA competitively inhibited [3H]CP55,940 binding in human CB1 (hCB1) cell membranes with a Ki value of 8.13 ,M (4.97,13.32 ,M, n=2). In human CB2 transfected (hCB2) HEK-293T cell membranes, 100 ,M ODA produced only a partial (42.5±7%) inhibition of [3H]CP55,940 binding. ODA stimulated [35S]GTP,S binding in a concentration-dependent manner (EC50=1.64 ,M (0.29,9.32 ,M), R2=0.99, n=4,9), with maximal stimulation of 188±9% of basal at 100 ,M. AEA stimulated [35S]GTP,S binding with an EC50 of 10.43 ,M (4.45,24.42 ,M, R2=1.00, n=3, 195±4% of basal at 300 ,M). Trans -oleamide (trans- ODA) failed to significantly stimulate [35S]GTP,S binding at concentrations up to 100 ,M. ODA (10 ,M)-stimulated [35S]GTP,S binding was reversed by the selective CB1 antagonist SR141716A (IC50=2.11 nM (0.32,13.77 nM), R2=1.00, n=6). The anatomical distribution of ODA-stimulated [35S]GTP,S binding in rat brain sections was indistinguishable from that of HU210. Increases of similar magnitude were observed due to both agonists in the striatum, cortex, hippocampus and cerebellum. ODA (10 ,M) significantly inhibited forskolin-stimulated cyclic AMP (cAMP) accumulation in mouse neuroblastoma N1E 115 cells (P=0.02, n=11). ODA-mediated inhibition was completely reversed by 1 ,M SR141716A (P<0.001, n=11) and was also reversed by pretreatment with 300 ng ml,1 pertussis toxin (P<0.001, n=6). These data demonstrate that ODA is a full cannabinoid CB1 receptor agonist. Therefore, in addition to allosteric modulation of other receptors and possible entourage effects due to fatty acid amide hydrolase inhibition, the effects of ODA may be mediated directly via the CB1 receptor. British Journal of Pharmacology (2004) 141, 253,262. doi:10.1038/sj.bjp.0705607 [source] | |||||||||||||