Martin Guy, Ferrier Bernard, Conjard Agnès, Martin Mireille, Nazaret Rémi, Boghossian Michelle, Saadé Fadi, Mancuso Claire, Durozard Daniel, Baverel Gabriel
Institut National de la Santé et de la Recherche Médicale, UMR 499, Animet, Faculté de Médecine RTH Laennec, Université Lyon 1, Rue G. Paradin, 69372 Lyon Cedex 08, France.
Biochem J. 2007 Jan 15;401(2):465-73. doi: 10.1042/BJ20061148.
Recent reports have indicated that 48-72 h of fasting, Type 1 diabetes and high-protein feeding induce gluconeogenesis in the small intestine of adult rats in vivo. Since this would (i) represent a dramatic revision of the prevailing view that only the liver and the kidneys are gluconeogenic and (ii) have major consequences in the metabolism, nutrition and diabetes fields, we have thoroughly re-examined this question in the situation reported to induce the highest rate of gluconeogenesis. For this, metabolically viable small intestinal segments from 72 h-fasted adult rats were incubated with [3-13C]glutamine as substrate. After incubation, substrate utilization and product accumulation were measured by enzymatic and NMR spectroscopic methods. Although the segments utilized [13C]glutamine at high rates and accumulated 13C-labelled products linearly for 30 min in vitro, no substantial glucose synthesis could be detected. This was not due to the re-utilization of [13C]glucose initially synthesized from [13C]glutamine. Arteriovenous metabolite concentration difference measurements across the portal vein-drained viscera of 72 h-fasted Wistar and Sprague-Dawley rats clearly indicated that glutamine, the main if not the only gluconeogenic precursor taken up, could not give rise to detectable glucose production in vivo. Therefore we challenge the view that the small intestine of the adult rat is a gluconeogenic organ.
最近的报告表明,禁食48 - 72小时、1型糖尿病和高蛋白喂养可在成年大鼠体内诱导小肠进行糖异生。由于这将(i)代表对仅肝脏和肾脏具有糖异生作用这一普遍观点的重大修正,并且(ii)在代谢、营养和糖尿病领域产生重大影响,我们在据报道诱导糖异生率最高的情况下对这个问题进行了全面重新审视。为此,将来自禁食72小时成年大鼠的具有代谢活性的小肠段与[3 - 13C]谷氨酰胺作为底物一起孵育。孵育后,通过酶法和核磁共振光谱法测量底物利用情况和产物积累。尽管这些小肠段在体外以高速率利用[13C]谷氨酰胺并在30分钟内线性积累13C标记的产物,但未检测到大量葡萄糖合成。这并非由于最初由[13C]谷氨酰胺合成的[13C]葡萄糖的再利用。对禁食72小时的Wistar和Sprague - Dawley大鼠门静脉引流内脏的动静脉代谢物浓度差异测量清楚地表明,所摄取的主要(如果不是唯一的)糖异生前体谷氨酰胺在体内无法产生可检测到的葡萄糖生成。因此,我们对成年大鼠小肠是糖异生器官这一观点提出质疑。