Whited K L, Thao D, Lloyd K C Kent, Kopin A S, Raybould H E
Department of Anatomy, Physiology, and Cell Biology, School of Vetinary Medicine, University of California, Davis School of Veterinary Medicine, Davis, CA 95616, USA.
Am J Physiol Gastrointest Liver Physiol. 2006 Jul;291(1):G156-62. doi: 10.1152/ajpgi.00569.2005. Epub 2006 Mar 30.
Cholecystokinin (CCK), acting at CCK1 receptors (CCK1Rs) on intestinal vagal afferent terminals, has been implicated in the control of gastrointestinal function and food intake. Using CCK1R(-/-) mice, we tested the hypothesis that lipid-induced activation of the vagal afferent pathway and intestinal feedback of gastric function is CCK1R dependent. In anesthetized CCK1R(+/+) ("wild type") mice, meal-stimulated gastric acid secretion was inhibited by intestinal lipid infusion; this was abolished in CCK1R(-/-) mice. Gastric emptying of whole egg, measured by nuclear scintigraphy in awake mice, was significantly faster in CCK1R(-/-) than CCK1R(+/+) mice. Gastric emptying of chow was significantly slowed in response to administration of CCK-8 (22 pmol) in CCK1R(+/+) but not CCK1R(-/-) mice. Activation of the vagal afferent pathway was measured by immunohistochemical localization of Fos protein in the nucleus of the solitary tract (NTS; a region where vagal afferents terminate). CCK-8 (22 pmol ip) increased neuronal Fos expression in the NTS of fasted CCK1R(+/+) mice; CCK-induced Fos expression was reduced by 97% in CCK1R(-/-) compared with CCK1R(+/+) mice. Intralipid (0.2 ml of 20% Intralipid and 0.04 g lipid), but not saline, gavage increased Fos expression in the NTS of fasted CCK1R(+/+) mice; lipid-induced Fos expression was decreased by 47% in CCK1R(-/-) compared with CCK1R(+/+)mice. We conclude that intestinal lipid activates the vagal afferent pathway, decreases gastric acid secretion, and delays gastric emptying via a CCK1R-dependent mechanism. Thus, despite a relatively normal phenotype, intestinal feedback in response to lipid is severely impaired in these mice.
胆囊收缩素(CCK)作用于肠道迷走神经传入末梢的CCK1受体(CCK1Rs),与胃肠功能及食物摄入的调控有关。我们利用CCK1R基因敲除(-/-)小鼠,验证了如下假说:脂质诱导的迷走神经传入通路激活及胃功能的肠道反馈是依赖CCK1R的。在麻醉的CCK1R基因野生型(+/+)小鼠中,肠内输注脂质可抑制进食刺激的胃酸分泌;而在CCK1R(-/-)小鼠中,此作用消失。通过核素闪烁扫描法在清醒小鼠中测量全蛋的胃排空情况,发现CCK1R(-/-)小鼠的胃排空速度显著快于CCK1R(+/+)小鼠。在CCK1R(+/+)小鼠中,给予CCK-8(22 pmol)可显著减慢食物的胃排空速度,但在CCK1R(-/-)小鼠中则无此作用。通过免疫组化定位孤束核(NTS;迷走神经传入终止的区域)中的Fos蛋白来检测迷走神经传入通路的激活情况。CCK-8(22 pmol腹腔注射)可增加禁食的CCK1R(+/+)小鼠孤束核中神经元Fos的表达;与CCK1R(+/+)小鼠相比,CCK诱导的Fos表达在CCK1R(-/-)小鼠中减少了97%。给予禁食的CCK1R(+/+)小鼠灌胃脂肪乳剂(0.2 ml 20%的脂肪乳剂和0.04 g脂质)而非生理盐水,可增加孤束核中Fos的表达;与CCK1R(+/+)小鼠相比,脂质诱导的Fos表达在CCK1R(-/-)小鼠中减少了47%。我们得出结论,肠内脂质通过依赖CCK1R的机制激活迷走神经传入通路,减少胃酸分泌并延迟胃排空。因此,尽管这些小鼠的表型相对正常,但它们对脂质的肠道反馈严重受损。