正常和营养不良小鼠血液和骨骼肌中的次黄嘌呤-鸟嘌呤磷酸核糖基转移酶活性。

J S Neerunjun, J Allsop, V Dubowitz
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引用次数: 4

摘要

1. 以[8(-14)C]次黄嘌呤为底物,5-磷酸基核糖1-焦磷酸为核糖5-磷酸供体,在正常和营养不良的129 ReJ和C57 BL/6J小鼠的红细胞血液和股四头肌提取物中测定了次黄嘌呤-鸟嘌呤磷酸化核糖转移酶(HGPRT)的活性。[8(-14)C]用高压电泳分离形成的肌苷单磷酸,用液体闪烁计数测定放射性。2. 在红细胞溶血液中,HGPRT活性在正常和营养不良的C57 BL/6J小鼠中相似,但在营养不良的C57 BL/6J小鼠中明显高于正常的129 ReJ小鼠。酶活性升高仅在临床严重感染的小鼠中观察到。3.在肌肉匀浆中,129 ReJ和C57 BL/6J小鼠的营养不良小鼠的HGPRT活性显著高于正常动物。酶活性与疾病的严重程度无关。4. 这表明红细胞的变化是继发于营养不良过程的,骨骼肌中HGPRT活性的升高可能与异常的能量代谢有关,可能通过单磷酸戊糖分流。
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Hypoxanthine--guanine phosphoribosyltransferase activity in blood and skeletal muscles of normal and dystrophic mice.

1. Hypoxanthine--guanine phosphoribosyltransferase (HGPRT) activity was measured in erythrocyte haemolysates and quadriceps muscle extracts of normal and dystrophic 129 ReJ and C57 BL/6J mice with [8(-14)C]hypoxanthine as substrate and 5-phosphorylribose 1-pyrophosphate as a ribose 5-phosphate donor. [8(-14)C]Inosine monophosphate formed was separated by high-voltage electrophoresis and radioactivity was measured by liquid-scintillation counting. 2. In erythrocyte haemolysates, HGPRT activity was similar in normal and dystrophic C57 BL/6J mice but was significantly higher in dystrophic than in normal 129 ReJ mice. Elevated enzyme activity was observed only in mice that were clinically severely affected. 3. In muscle homogenates, HGPRT activity was significantly higher in dystrophic than in normal animals of both 129 ReJ and C57 BL/6J mice. Enzyme activity was not related to the severity of the disease. 4. It is suggested that changes in erythrocytes are secondary to the dystrophic process and that elevated HGPRT activity in skeletal muscle may be related to abnormal energy metabolism, possibly via the pentose monophosphate shunt.

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Proceedings of the Fifth Meeting of the International Society of Hypertension, Paris, 12-14 June 1978. Brain catecholamines and catecholamine-synthesizing enzymes in renovascular hypertension in the rat. Enhanced hypothalamic noradrenaline biosynthesis in Goldblatt I renovascular hypertension. Definitive evidence for renin in rat brain by affinity chromatographic separation from protease. Renal release of active and inactive renin in essential and renovascular hypertension.
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