Effect of sialoadenectomy and salivary gland extracts on gastrointestinal mucosal growth and gastrin levels in the rat.

Skinner, Karolina; Soper, B. D.; Tepperman, Barry L.

doi:10.1113/jphysiol.1984.sp015227

Cited by 51 publications

(23 citation statements)

References 28 publications

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“…Sialoadenectomy was performed under pentobarbitone anaesthesia (60mg kg-', i.p.) by removal of the submandibularsublingual gland complexes after the ducts were ligated as previously described (Skinner & Tepperman, 1981;Skinner et al, 1984). SALX and sham-operated animals were administered an antibiotic (Pen-Di-Strep 0.1 ml, i.m.)…”

Section: Animal Preparationmentioning

confidence: 99%

Effect of nitric oxide on integrity, blood flow and cyclic GMP levels in the rat gastric mucosa: modulation by sialoadenectomy

Tripp

Tepperman

1995

British J Pharmacology

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The effects of the nitrosothiol, S‐nitroso N‐acetylpenicillamine (SNAP) which liberates nitric oxide (NO), on ethanol‐mediated gastric damage, blood flow and cyclic GMP levels in siaoloadenectomized (SALX) rats have been investigated. Intraluminal instillation of ethanol (5–50% w/v) dose‐dependently induced haemorrhagic damage and decreased NO synthase activity in the gastric mucosa. Both the extent of mucosal damage and inhibition of NO synthase activity were exacerbated in SALX rats. Epidermal growth factor administration (5 and 10 μg kg−1, s.c.) reduced mucosal damage but did not restore NO synthase activity in ethanol‐treated SALX rats. SNAP infusion (0.01‐1.0 μg kg−1 min−1, i.v.) attenuated haemorrhagic damage in ethanol‐treated rats. The reduction in mucosal damage was significantly greater in SALX rats. SNAP administration also caused an increase in gastric mucosal blood flow and cyclic GMP levels in control rats and both responses were augmented in SALX animals. These data suggest that SALX is associated with increases in mucosal susceptibility to ethanol‐mediated damage and reduces mucosal NO synthase activity. Epidermal growth factor does not appear to influence mucosal NO synthase in ethanol‐treated rats. Furthermore, SALX augments the responsiveness of the gastric mucosa to NO administration. Therefore, factors from the salivary glands influence gastric NO formation and mucosal responsiveness to a NO donor.

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Section: Animal Preparationmentioning

confidence: 99%

Effect of nitric oxide on integrity, blood flow and cyclic GMP levels in the rat gastric mucosa: modulation by sialoadenectomy

Tripp

Tepperman

1995

British J Pharmacology

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“…Cell viability was always at least 90%, and the cell concentration for inoculation was 4.5 x 10 7 viable cells/ml. SGE was prepared by the method of Skinner et al (6). One hundred pairs of submaxillary glands were harvested from adult male mice and homogenized with a manual tissue homogenizer and 0.3 ml of 0.2% (w/v) soybean trypsin inhibitor (Sigma Chemical Co., St. Louis, MO, USA) and 7.7 ml PBS/g gland were added at 4 o C. The homogenate was centrifuged at 20,000 g for 30 min at 4 o C and the supernatant was stored at -30 o C until use.…”

Section: Cells Pre-incubated With a Submaxillary Gland Extract (Sge)mentioning

confidence: 99%

Effect of a submaxillary gland extract on Ehrlich tumor growth in mice

Weill

Frussa‐Filho

Bonamin

1999

Braz J Med Biol Res

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Ablation of host submaxillary glands modifies Ehrlich tumor growth and tumor-infiltrating leukocytes, possibly by modifications in the serum level of growth factors produced by this gland. To extend this research, 7-month-old male EPM-1 mice (N = 30) were divided into two groups: 1) inoculated with tumor cells previously incubated with submaxillary salivary gland extract (SGE) in PBS for 30 min at 37%; 2) inoculated with tumor cells previously incubated with PBS, under the same conditions. Animals were inoculated into the footpad with 40 µl of a suspension containing 4.5 x 10 7 tumor cells/ml, and footpad thickness was measured daily for 10 days. Sections and smears of tumor cells were prepared from the tumor mass to determine mitosis frequency, percent of tumor cells immunopositive to nerve (NGF) and epidermal (EGF) growth factors and percent of tumor-infiltrating leukocytes. The incubation of tumor cells with SGE produced a tumor reduction of about 30% in size (P<0.01). This effect was not related to loss of cell viability during incubation, but a 33% increase (P<0.05) in the percentage of dead or dying tumor cells and a 15% increase in the percent of NGF/EGF-positive tumor cells (P<0.01) were observed in vivo at the end of experiment. Tumor-infiltrating lymphocytes and mitosis frequency did not differ between groups. These data suggest a direct effect of factors present in SGE on tumor cells, which induce degeneration of tumor cells. Correspondence

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“…Removal of salivary glands (the major intraluminal source of EGF) in rats results in atrophy of gastric mucosa (17) and a delay in healing ofgastric and duodenal ulcerations that can be reversed by treating the animals with either oral or parenteral EGF (18). These studies imply an important physiological role for EGF in gastric mucosal growth.…”

Section: Introductionmentioning

confidence: 99%

Localization of transforming growth factor alpha and its receptor in gastric mucosal cells. Implications for a regulatory role in acid secretion and mucosal renewal.

Beauchamp¹,

Barnard²,

McCutchen³

et al. 1989

J. Clin. Invest.

229

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Transforming growth factor a (TGFa) shares with epidermal growth factor (EGF) structural homology (35%), a common cell-surface membrane receptor (TGFa/EGF receptor), and a nearly identical spectrum of biological activity, including inhibition of gastric acid secretion. Herein, we report expression of TGFa mRNA in normal gastric mucosa of the adult guinea pig, rat, and dog. TGFa mRNA was also detected in matched surgically resected gastric mucosa and adjacent gastric carcinoma from 10 patients, and in gastric mucosa adjacent to a benign ulcer from an additional patient. TGFa protein was quantitated by radioimmunoassay and was present in tumor and adjacent mucosa. TGFa/EGF receptor mRNA was also detected in gastric mucosa from all species studied. Localization of TGFa and TGFa/EGF receptor mRNA expression was examined in samples of unfractionated guinea pig gastric mucosa and from chief cell-enriched and parietal cell-enriched fractions. All samples exhibited TGFa and TGFa/EGF receptor expression. The TGFa signal was greatest in the parietal cell fraction (5.8-fold increase), but was also enhanced in the chief cell fraction (1.9-fold increase) relative to the unfractionated gastric mucosa. Like TGFa expression, TGFa/EGF receptor mRNA expression was most intense in the parietal cellenriched fraction (7.8-fold increase), but was also increased in the chief cell-enriched fraction (2.7-fold increase) relative to the unfractionated guinea pig gastric mucosa. We conclude that TGFa and TGFa/EGF receptor genes are expressed in normal adult mammalian gastric mucosa. These findings, when interpreted in light of described actions of TGFa and EGF, provide evidence that local production of TGFa could play an important role in the regulation of acid secretion and mucosal renewal in the stomach.

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Effect of sialoadenectomy and salivary gland extracts on gastrointestinal mucosal growth and gastrin levels in the rat.

Cited by 51 publications

References 28 publications

Effect of nitric oxide on integrity, blood flow and cyclic GMP levels in the rat gastric mucosa: modulation by sialoadenectomy

Effect of nitric oxide on integrity, blood flow and cyclic GMP levels in the rat gastric mucosa: modulation by sialoadenectomy

Effect of a submaxillary gland extract on Ehrlich tumor growth in mice

Localization of transforming growth factor alpha and its receptor in gastric mucosal cells. Implications for a regulatory role in acid secretion and mucosal renewal.

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