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通过细胞容积调节机制控制肝脏氮代谢和谷胱甘肽释放。

Control of hepatic nitrogen metabolism and glutathione release by cell volume regulatory mechanisms.

作者信息

Hüssinger D, Lang F, Bauers K, Gerok W

机构信息

Medizinische Universitätsklinik Freiburg, Federal Republic of Germany.

出版信息

Eur J Biochem. 1990 Nov 13;193(3):891-8. doi: 10.1111/j.1432-1033.1990.tb19414.x.

Abstract
  1. Urea synthesis was studied in isolated perfused rat liver during cell volume regulatory ion fluxes following exposure of the liver to anisotonic perfusion media. Lowering of the osmolarity in influent perfusate from 305 mOsm/l to 225 mOsm/l (by decreasing influent [NaCl] by 40 mmol/l) led to an inhibition of urea synthesis from NH4Cl (0.5 mmol/l) by about 60% and a decrease of hepatic oxygen uptake by 0.43 +/- 0.03 mumol g-1 min-1 [from 3.09 +/- 0.13 mumol g-1 min-1 to 2.66 +/- 0.12 mumol g-1 min-1 (n = 9)]. The effects on urea synthesis and oxygen uptake were observed throughout hypotonic exposure (225 mOsm/l). They persisted although volume regulatory K+ efflux from the liver was complete within 8 min and were fully reversible upon reexposure to normotonic perfusion media (305 mOsm/l). A 42% inhibition of urea synthesis from NH4Cl (0.5 mmol/l) during hypotonicity was also observed when the perfusion medium was supplemented with glucose (5 mmol/l). Urea synthesis was inhibited by only 10-20% in livers from fed rats, and was even stimulated in those from starved rats when an amino acid mixture (twice the physiological concentration) plus NH4Cl (0.2 mmol/l) was infused. 2. The inhibition of urea synthesis from NH4Cl (0.5 mmol/l) during hypotonicity was accompanied by a threefold increase of citrulline tissue levels, a 50-70% decrease of the tissue contents of glutamate, aspartate, citrate and malate, whereas 2-oxoglutarate, ATP and ornithine tissue levels, and the [3H]inulin extracellular space remained almost unaltered. Further, hypotonic exposure stimulated hepatic glutathione (GSH) release with a time course roughly paralleling volume regulatory K+ efflux. NH4Cl stimulated lactate release from the liver during hypotonic but not during normotonic perfusion. In the absence of NH4Cl, hypotonicity did not significantly affect the lactate/pyruvate ratio in effluent perfusate. With NH4Cl (0.5 mmol/l) present, the lactate/pyruvate ratio increased from 4.3 to 8.2 in hypotonicity, whereas simultaneously the 3-hydroxybutyrate/acetoacetate ratio slightly, but significantly decreased. 3. Addition of lactate (2.1 mmol/l) and pyruvate (0.3 mmol/l) to influent perfusate did not affect urea synthesis in normotonic perfusions, but completely prevented the inhibition of urea synthesis from NH4Cl (0.5 mmol/l) induced by hypotonicity. Restoration of urea production in hypotonic perfusions by addition of lactate and pyruvate was largely abolished in the presence of 2-cyanocinnamate (0.5 mmol/l). Addition of 3-hydroxybutyrate (0.5 mmol/l), but not of acetoacetate (0.5 mmol/l) largely reversed the hypotonicity-induced inhibition of urea synthesis from NH4Cl.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 在将肝脏暴露于非等渗灌注介质后,于分离灌注的大鼠肝脏中研究尿素合成过程中的细胞容积调节离子通量。将流入灌注液的渗透压从305 mOsm/l降至225 mOsm/l(通过将流入液中[NaCl]降低40 mmol/l),导致由NH4Cl(0.5 mmol/l)合成尿素受到约60%的抑制,肝脏氧摄取量降低0.43±0.03 μmol g-1 min-1[从3.09±0.13 μmol g-1 min-1降至2.66±0.12 μmol g-1 min-1(n = 9)]。在整个低渗暴露(225 mOsm/l)过程中均观察到对尿素合成和氧摄取的影响。尽管肝脏的容积调节性K+外流在8分钟内完成,但这些影响持续存在,并且在重新暴露于等渗灌注介质(305 mOsm/l)后完全可逆。当灌注介质中添加葡萄糖(5 mmol/l)时,低渗状态下由NH4Cl(0.5 mmol/l)合成尿素也受到42%的抑制。喂食大鼠肝脏中的尿素合成仅受到10 - 20%的抑制,而当输注氨基酸混合物(两倍生理浓度)加NH4Cl(0.2 mmol/l)时,饥饿大鼠肝脏中的尿素合成甚至受到刺激。2. 低渗状态下由NH4Cl(0.5 mmol/l)合成尿素受到抑制的同时,瓜氨酸组织水平增加了三倍,谷氨酸、天冬氨酸、柠檬酸和苹果酸的组织含量降低了50 - 70%,而2-氧代戊二酸、ATP和鸟氨酸的组织水平以及[3H]菊粉细胞外间隙几乎未改变。此外,低渗暴露刺激肝脏谷胱甘肽(GSH)释放,其时间进程大致与容积调节性K+外流平行。在低渗灌注期间NH4Cl刺激肝脏释放乳酸,但在等渗灌注期间不刺激。在没有NH4Cl的情况下,低渗状态对流出灌注液中乳酸/丙酮酸比值没有显著影响。存在NH4Cl(0.5 mmol/l)时,低渗状态下乳酸/丙酮酸比值从4.3增加到8.2,而同时3-羟基丁酸/乙酰乙酸比值略有但显著降低。3. 向流入灌注液中添加乳酸(2.1 mmol/l)和丙酮酸(0.3 mmol/l)在等渗灌注中不影响尿素合成,但完全防止了低渗状态诱导的由NH4Cl(0.5 mmol/l)合成尿素的抑制。在存在2-氰基肉桂酸(0.5 mmol/l)的情况下,通过添加乳酸和丙酮酸恢复低渗灌注中的尿素生成在很大程度上被消除。添加3-羟基丁酸(0.5 mmol/l)而不是乙酰乙酸(0.5 mmol/l)在很大程度上逆转了低渗状态诱导的由NH4Cl合成尿素的抑制。(摘要截断于400字)

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