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1. |
New insights on the mechanism of the alcohol-induced increase in portal blood flow |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 1-9
H. Orrego,
F. J. Carmichael,
Y. Israel,
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摘要:
Acute administration of ethanol increases portal blood flow by 40–60%. This increase in blood flow compensates for the increase in O2consumption that follows alcohol intake and may play a protective role against hypoxic hepatocellular necrosis. We have investigated the mechanism of this hemodynamic effect of ethanol in the rat using the labeled microsphere technique. We ruled out a direct role of systemic glucagon and of acetaldehyde in mediating the increase in portal flow. However, the increase in flow is maximal at a blood ethanol concentration of 3.5 mM, corresponding to that required to achieve theVmaxof alcohol dehydrogenase, and is suppressed by 4-methylpyrazole, an inhibitor of alcohol dehydrogenase. Alcohol ingestion results in zonal liver hypoxia and in increases in acetate, both of which have been shown to increase the levels of adenosine, a potent vasodilator, in blood and tissues. Ethanol produces a 400% increase in arterial adenosine. Adenosine infusion leads to a dose-dependent increase in portal blood flow of up to 100%, an effect that is suppressed by administration of 8-phenyltheophylline, an antagonist of adenosine at A1and A2receptors. Similarly, the ethanol-induced increase in portal blood flow is fully suppressed by 8-phenyltheophylline. In conclusion, adenosine appears to play an important role in the mechanism by which ethanol increases portal blood flow.
ISSN:0008-4212
DOI:10.1139/y88-001
出版商:NRC Research Press
年代:1988
数据来源: NRC
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2. |
Role of inositol phospholipid hydrolysis in the initiation of agonist-induced contractions of rat uterus: effects of domination by 17β-estradiol and progesterone |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 10-17
A. L. Ruzycky,
D. J. Crankshaw,
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摘要:
The role of inositol phospholipid (IP) hydrolysis in agonist-mediated contractility was examined in rat uterine smooth muscle by comparing carbachol-, oxytocin-, and PGF2αmediated [3H]IP accumulation and tension generation. In both estrogen- and progesterone-dominated uteri, all three agonists exhibited dose-dependent contractile responses. Agonist potencies (EC50values) for eliciting [3H]IP accumulation or contractile responses were found to be very similar and did not change significantly between hormonal states. Maximal responses of agonist-mediated [3H]IP accumulation and tension generation were significantly affected by the endocrine state of the uterus and were dependent on the agonist examined. Maximal carbachol- and PGF2α-induced [3H]IP accumulation were found to be elevated in estrogen-dominated relative to progesterone-dominated uteri, whereas maximal forces generated by these two agonists were smaller in progesterone-dominated relative to estrogen-dominated tissues. Oxytocin-induced responses did not differ between hormonal states. To determine whether these differences between [3H]IP accumulation and contractility responses could be attributed to changes in receptor-mediated signal transduction mechanisms, receptor expression and coupling to phospholipase C were studied. Myometrial muscarinic and oxytocin receptors assessed by radioligand binding were found to have three- to four-fold greater capacities in estrogen-dominated than in progesterone-dominated uteri without significant changes in agonist affinities. Agonist-mediated [3H]IP accumulation was potently inhibited by both pertussis and cholera toxins in both hormonal states. These experiments show that estrogen- and progesterone-dominated environments regulate both uterine excitability and contractility and that the mechanisms of this regulation are complex and dependent on the agonist system stimulated.
ISSN:0008-4212
DOI:10.1139/y88-002
出版商:NRC Research Press
年代:1988
数据来源: NRC
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3. |
Adrenomedullary origin of the hindquarter vasodilation during the transposition response of the rat |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 18-21
S. Sakata,
J. Iriuchijima,
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摘要:
Transposing a rat from the home cage to a new cage produces a cardiovascular response (transposition response) characterized by an increase in hindquarter blood flow with unchanged systemic arterial pressure. Arterial blood samples were collected from rats before and during this response for radioenzymatic assay of catecholamines. During the transposition response, the concentration of adrenaline and noradrenaline in plasma increased about six- and two-fold, respectively. Ablation of the adrenal medulla prevented these changes in plasma catecholamine concentration. Constant i.v. infusion of adrenaline, at rates producing a hindquarter flow approximately matching that observed during the transposition response, evoked an increase in plasma adrenaline concentration also approximately matching the increase observed during the transposition response. It is concluded that the increase in plasma adrenaline secreted from the adrenal medulla is the main cause of the increase in hindquarter blood flow in the transposition response.
ISSN:0008-4212
DOI:10.1139/y88-003
出版商:NRC Research Press
年代:1988
数据来源: NRC
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4. |
Simultaneous and independent release of vasopressin and oxytocin in the rat |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 22-26
Norman W. Kasting,
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摘要:
The relative dependence or independence of the secretion of the neurohypophysial hormones, arginine vasopressin and oxytocin, was investigated using a wide variety of stimuli reported to cause the secretion of one or the other hormone. Differences in species, animal preparations, sampling techniques, assays, and other factors make comparison of many previous studies difficult. The aim of this study was to overcome these problems by using the same methodology, animal species, and assays to compare vasopressin and oxytocin release. To further strengthen the analysis, determinations of vasopressin and oxytocin were done in the same blood samples. The results demonstrated that during simultaneous release of both hormones, vasopressin is released in greater proportion following restraint stress, hemorrhage, isotonic hypovolemia, and nicotine, whereas oxytocin is released in greater proportion following endotoxin or hypertonic saline. Vasopressin was released without oxytocin following diethylstilbestrol. Oxytocin was released without concomitant vasopressin release following exercise, hypothermia, hyperthermia, labour, and lactation. Neither oxytocin nor vasopressin release was observed following thyroid-releasing hormone or insulin-induced hypoglycemia. These data illustrate the marked flexibility of the hypothalamo-neurohypophysial system that regulates secretion of vasopressin and oxytocin.
ISSN:0008-4212
DOI:10.1139/y88-004
出版商:NRC Research Press
年代:1988
数据来源: NRC
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5. |
The effects of neomycin on membrane properties and discharge activity of an isolated sensory neuron |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 27-31
Patrick N. Nation,
Sheldon H. Roth,
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摘要:
The effects of neomycin sulfate were examined upon the discharge activity and electrical membrane properties of an isolated invertebrate sensory neuron, the crayfish stretch receptor neuron. Neomycin depressed cell discharge activity in a concentration-dependent manner over the concentration range of 0.01–1.0 mM. Significant concentration-related increases were observed in the resting membrane potential and the width of the orthodromic action potential. There was a significant concentration-dependent decrease in the fast rising phase of the antidromic action potential. Significant changes also were observed in other electrical properties such as membrane resistance, but these were found not to be concentration related. The most significant change was membrane hyperpolarization, which could account for the depression of cell discharge activity. The observed changes are consistent with a neomycin-induced change in the membrane potassium conductance. It is proposed that the neural effect of neomycin is a selective interaction with the neuronal membrane phospholipids.
ISSN:0008-4212
DOI:10.1139/y88-005
出版商:NRC Research Press
年代:1988
数据来源: NRC
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6. |
BAY-K-8644-stimulated amylase secretion from pancreatic acinar cells |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 32-37
Seymour Heisler,
Diane Desjardins,
Marthe Belles-Isles,
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摘要:
Pancreatic acinar cells do not contain depolarization-sensitive calcium channels. Nonetheless, in the current study, the calcium channel activator, BAY-K-8644, was found to stimulate a time- and concentration-dependent increase in the spontaneous release of amylase. Secretion was dependent on the presence of extracellular calcium in the incubation medium. Racemic BAY-K-8644 and (or) itsS(−)optical isomer did not enhance the secretory response to either carbachol or cholecystokinin octapeptide; however, when co-applied with either phorbol ester, vasoactive intestinal peptide, or forskolin, they potentiated amylase secretion. Nifedipine and theR(+)isomer of BAY-K-8644, which are both calcium channel antagonists, did not alter basal or forskolin-stimulated amylase secretion, and [3H]nitrendipine did not bind to acinar cell membranes. Neither atropine nor dibutyryl cGMP, inhibitors of cholinergic and cholecystokininergic receptors, respectively, affected BAY-K-8644-induced amylase secretion. While BAY-K-8644 stimulated concentration-dependent cGMP synthesis in acinar cells, it had no effect on basal or forskolin-stimulated cAMP formation. The data suggest that BAY-K-8644 may bind to acinar cell sites that are not functional calcium channel proteins but are coupled nevertheless to the secretory response, and that calcium channel antagonists do not bind to these sites. The mechanism of the secretagogue action of BAY-K-8644 remains to be elucidated.
ISSN:0008-4212
DOI:10.1139/y88-006
出版商:NRC Research Press
年代:1988
数据来源: NRC
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7. |
Opioidergic control of luteinizing hormone secretion in the female rabbit: influence of age on the response to naloxone |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 38-42
E. V. YoungLai,
M. Wilkinson,
N. Thompson,
A. Byrne,
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摘要:
To examine the role of opioid neurons on luteinizing hormone (LH) secretion in the female rabbit, we determined LH release at timed intervals after naloxone administration to rabbits aged 25–150 days. The LH response to naloxone (10 mg/kg) was not significantly elevated until day 43 when LH rose 76–113% above basal levels at 40–80 min. In 56-day-old females the corresponding increase was 160% at 15 min and in 65- to 67-day-olds it was 154%. From 70 to 80 days of age the LH response was blunted and no significant elevations could be elicited. By contrast, naloxone-induced LH increases were again evident when rabbits were older than 100 days. At all ages no significant change in FSH concentrations was observed. In the adult females, naloxone at 2.5, 5, and 10 mg/kg caused increases in LH secretion which occasionally were high enough to induce ovulation as exemplified by elevated serum progesterone 4 days later. These data suggest that opioid peptides may be involved in the prepubertal rise in LH and in the normal inhibition of adult secretion in the female rabbit.
ISSN:0008-4212
DOI:10.1139/y88-007
出版商:NRC Research Press
年代:1988
数据来源: NRC
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8. |
Bradykinin stimulates a rise in cytosolic calcium in renal glomerular mesangial cells via a pertussis toxin insensitive pathway |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 43-48
S. Kremer,
P. Harper,
R. Hegele,
K. Skorecki,
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摘要:
Bradykinin elicits a complex response in the renal glomerulus which includes a reduction in the glomerular capillary ultrafiltration coefficient. To elucidate the biochemical mechanism of this response, we investigated calcium signalling in rat renal glomerular mesangial cells in culture using the calcium-sensitive fluorescent dye, Indo-1. Bradykinin was found to cause a concentration-dependent transient rise in cytosolic free calcium followed by a sustained slower secondary rise. The bradykinin response persisted with acute removal of extracellular calcium using EGTA, indicating that calcium entry from outside the cell did not mediate this primary response. Prolonged exposure to EGTA, which reduced intracellular stores, eliminated the calcium response to bradykinin but not to vasopressin, indicating differential sensitivity to intracellular calcium stores of these two hormonal responses. In agreement, prior stimulation with vasopressin significantly attenuated the response to bradykinin, but the converse did not occur. Aluminum fluoride and pertussis toxin were used to investigate the possible involvement of a guanyl nucleotide regulatory protein in signal transduction. Aluminum fluoride induced a transient rise in cytosolic calcium that was abrogated by prior exposure of the cells to pertussis toxin. This demonstrates the effectiveness of pertussis toxin and the presence of a calcium-signalling pathway susceptible to pertussis toxin in these cells. In contrast, the responses to bradykinin and vasopressin were unaffected by pertussis toxin. We conclude that bradykinin stimulates release of calcium from intracellular stores in glomerular mesangial cells via a pertussis toxin insensitive pathway. This mesangial response provides a direct biochemical basis for the bradykinin-induced fall in glomerular capillary ultrafiltration coefficient which has been observed in vivo.
ISSN:0008-4212
DOI:10.1139/y88-008
出版商:NRC Research Press
年代:1988
数据来源: NRC
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9. |
Myosin light chain phosphorylation and contractile performance of human skeletal muscle |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 49-54
D. S. Stuart,
M. D. Lingley,
R. W. Grange,
M. E. Houston,
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摘要:
Twitch tension and maximal unloaded velocity of human knee extensor muscles were studied under conditions of low phosphate content of the phosphorylatable light chains (P-light chains) of myosin and elevated phosphate content, following a 10-s maximal voluntary isometric contraction (MVC). After the MVC, twitch tension was significantly potentiated, with greater potentiation observed at a shorter muscle length (p < 0.05). The MVC was associated with at least a twofold increase in phosphate content of the fast (LC2F) and two slow (LC2S and LC2S′) P-light chains, but this increase was unrelated to muscle length. No significant differences in knee extension velocity were observed between conditions where P-light chains had low or elevated phosphate content. Positive but nonsignificant correlations were noted between the extent of twitch potentiation and phosphate content of individual P-light chains as well as the percentage of type II muscle fibres in vastus lateralis muscle. No significant relationships were determined for myosin light chain kinase activity and either P-light chain phosphorylation or type II fibre percentage. These data suggest that, unlike other mammalian fast muscles, P-light chain phosphorylation of mixed human muscles is not strongly associated with altered contractile performance.
ISSN:0008-4212
DOI:10.1139/y88-009
出版商:NRC Research Press
年代:1988
数据来源: NRC
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10. |
Degradation and conversion of somatostatin in normal and diabetic ratsin vivoandin vitro |
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Canadian Journal of Physiology and Pharmacology,
Volume 66,
Issue 1,
1988,
Page 55-60
Michiyo Seno,
Kinsuke Tsuda,
Norikazu Kitano,
Jun Takeda,
Hirofumi Fukumoto,
Gyohan Koh,
Hiroo Imura,
Tomohiko Taminato,
Yutaka Seino,
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摘要:
Plasma somatostatin-like immunoreactivity in the portal and jugular veins of streptozotocin diabetic rats was compared with that in normal control rats. In the diabetic group, somatostatin levels in the portal (p < 0.05) and jugular (p < 0.01) veins were both elevated compared with those in the control group. Moreover, the degree of elevation was greater in the jugular vein than in the portal vein. To further investigate the role of the liver in the clearance of somatostatin-28in vivo, 2 μg of somatostatin-28 was administered as a bolus into the external jugular vein of intact and functionally hepatectomized rats. The mean half-time of somatostatin-28 was significantly longer in intact diabetic rats than in controls (p < 0.05). The functional hepatectomy did not cause a significant difference in the half-time in diabetic rats but made it longer in control rats. These results suggest that the longer half-time of somatostatin-28 in diabetic ratsin vivois due to its slower hepatic clearance. The hepatic clearance of somatostatin-28 and somatostatin-14 was further studiedin vitrousing a recirculating liver perfusion method. The hepatic clearance of 1.2 nM of either somatostatin-28 or somatostatin-14 was significantly lower in diabetic rats than in controls (p < 0.01). This indicates that elevated plasma somatostatin levels in diabetic rats are caused at least in part by decreased hepatic clearance of somatostatin. Gel chromatography of plasma samples obtained 0.5 and 4 min after the somatostatin-28 injection into intact, hepatectomized, and nephrectomized rats showed two major peaks: one compatible with somatostatin-28 and the other compatible with somatostatin-14 in elution position, in both diabetic and control rats. When somatostatin-28 was added to perfusatein vitro, however, gel chromatography failed to demonstrate the second peak was compatible with somatostatin-14 even after 30 min of recirculating perfusion. Gel chromatography of plasma samples obtained 5 and 30 min after incubation of somatostatin-28 showed two major peaks: one compatible with somatostatin-28 and the other compatible with somatostatin-14 in both diabetic and control rats. These results suggest that the conversion of somatostatin-28 to somatostatin-14 occurs mainly in plasmain vivo.
ISSN:0008-4212
DOI:10.1139/y88-010
出版商:NRC Research Press
年代:1988
数据来源: NRC
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