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离体灌注大鼠肝脏尿素合成调节因子的分析。I. 以氨和谷氨酰胺为氮源的尿素合成

Analysis of regulatory factors for urea synthesis by isolated perfused rat liver. I. Urea synthesis with ammonia and glutamine as nitrogen sources.

作者信息

Saheki T, Katunuma N

出版信息

J Biochem. 1975 Mar;77(3):659-69. doi: 10.1093/oxfordjournals.jbchem.a130768.

Abstract

Urea synthesis was studied using the isolated liver perfusion with ammonium cholride and glutamine as nitrogen sources. The rate of urea formation increases with ammonium cholorde concentration up to 5mM, and the rate remained constant in the range between 5 and 20mM of ammonium chloride as the substrate. The concentration of ammonia in the medium to support the half-maximum velocity of urea formation was 0.7mM. The rate of urea formation was stimulated by the addition of 2.5mM ornithine, and the greater part of the ornithine which was taken up into the liver was accumulated as citrulline in the presence of ammonia. A considerable accelerating effect of N-acetylglutamate on the synthetic rate was observed, but a rather high concentration of N-acetylglutamate was required in order to obtain the maximum effect possibly, because its permeability into liver cells may be limited. A marked additive effect on the rate of urea formation was observed with the combined addition of ornithine and N-acetylglutamate. The metabolic conversion of glutamine nitrogen to urea in the perfused rat liver and the effect of several compounds which stimulated urea synthesis with ammonia were further examined. The process of conversion of glutamine nitrogen to urea might be composed of the following three steps. In the first lag phase, a small amount of glutamine was removed from the medium. In the second stage, the glutamine level decreased rapidly and ammonia was accumulated in the perfusate. The third stage was a period in which glutamine concentration remained at a constant low level, and the accumulated ammonia was rapidly conversed to urea. The rate of urea formation in this third stage was found to be much higher than that with ammonia as the substrate. The maximum rate of glutamine removal was obtained at pH 7.7 of the perfusate and at a concentration of 10mM glutamine. Urea formation with glutamine was also stimulated by the addition of ornithine, malate, or N-acetylglutamate, which had accelerating effects on the urea synthesis with ammonia. This stimulation was due to an effective conversion of ammonia to urea, but no change in the rate of removal glutamine was obtained.

摘要

以氯化铵和谷氨酰胺作为氮源,采用离体肝脏灌注法研究尿素合成。随着氯化铵浓度增加至5mM,尿素生成速率升高;当氯化铵作为底物浓度在5至20mM范围内时,速率保持恒定。支持尿素生成半最大速度的培养基中氨浓度为0.7mM。添加2.5mM鸟氨酸可刺激尿素生成速率,在有氨存在的情况下,肝脏摄取的大部分鸟氨酸以瓜氨酸形式积累。观察到N-乙酰谷氨酸对合成速率有显著的促进作用,但可能需要相当高浓度的N-乙酰谷氨酸才能获得最大效果,因为其进入肝细胞的通透性可能有限。同时添加鸟氨酸和N-乙酰谷氨酸对尿素生成速率有明显的相加作用。进一步研究了灌注大鼠肝脏中谷氨酰胺氮向尿素的代谢转化以及几种用氨刺激尿素合成的化合物的作用。谷氨酰胺氮向尿素的转化过程可能由以下三个步骤组成。在第一个延迟阶段,少量谷氨酰胺从培养基中被去除。在第二阶段,谷氨酰胺水平迅速下降,氨在灌注液中积累。第三阶段是谷氨酰胺浓度保持在恒定低水平的时期,积累的氨迅速转化为尿素。发现该第三阶段的尿素生成速率远高于以氨作为底物时的速率。在灌注液pH 7.7和谷氨酰胺浓度为10mM时获得谷氨酰胺去除的最大速率。添加鸟氨酸、苹果酸或N-乙酰谷氨酸也可刺激谷氨酰胺生成尿素,这些物质对用氨合成尿素有促进作用。这种刺激是由于氨有效转化为尿素,但谷氨酰胺去除速率没有变化。

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