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一种用于过氧化物酶体β氧化的发光测定法。禁食和链脲佐菌素诱导的糖尿病对过氧化物酶体β氧化的影响。

A luminometric assay for peroxisomal beta-oxidation. Effects of fasting and streptozotocin-diabetes on peroxisomal beta-oxidation.

作者信息

Osmundsen H, Brodal B, Hovik R

机构信息

Department of Physiology and Biochemistry, Dental School, University of Oslo, Norway.

出版信息

Biochem J. 1989 May 15;260(1):215-20. doi: 10.1042/bj2600215.

Abstract
  1. A luminometric assay for acyl-CoA oxidase activity is described. The assay uses the luminol/microperoxidase system to monitor continuously acyl-CoA-dependent generation of H2O2. The assay is rapid, convenient, and lends itself to automation with an LKB 1251 luminometer. The assay is extremely sensitive, requiring at the most 10 micrograms of liver-homogenate protein per assay. 2. The assay can also be used to measure other oxidases, e.g. glycollate oxidase (EC 1.1.3.15), D-aspartate oxidase (EC 1.4.3.1) and urate oxidase (EC 1.7.3.3), the only modification being substitution of substrates to appropriate concentration. 3. With rat liver homogenates, spectrophotometrically measured rates of palmitoyl-CoA-dependent NAD+ reduction and acyl-CoA oxidase activity [Hryb & Hogg (1979) Biochem. Biophys. Res. Commun. 87, 1200-1206] was generally found in good agreement with luminometrically measured acyl-CoA oxidase activity. 4. With liver homogenates from streptozotocin-diabetic rats, however, rates of palmitoyl-CoA-dependent NAD+ reduction were consistently lower than the corresponding acyl-CoA oxidase activity. This difference was most marked with respect to luminometrically assayed acyl-CoA oxidase activity.
摘要
  1. 本文描述了一种用于测定酰基辅酶A氧化酶活性的发光测定法。该测定法使用鲁米诺/微过氧化物酶系统来连续监测酰基辅酶A依赖性过氧化氢的生成。该测定法快速、方便,并且适合使用LKB 1251发光计进行自动化操作。该测定法极其灵敏,每次测定最多需要10微克肝脏匀浆蛋白。2. 该测定法还可用于测量其他氧化酶,例如乙醇酸氧化酶(EC 1.1.3.15)、D-天冬氨酸氧化酶(EC 1.4.3.1)和尿酸氧化酶(EC 1.7.3.3),唯一的改动是将底物替换为适当浓度。3. 对于大鼠肝脏匀浆,通过分光光度法测定的棕榈酰辅酶A依赖性NAD⁺还原速率和酰基辅酶A氧化酶活性[Hryb & Hogg (1979) Biochem. Biophys. Res. Commun. 87, 1200 - 1206]通常与通过发光法测定的酰基辅酶A氧化酶活性高度一致。4. 然而,对于链脲佐菌素诱导的糖尿病大鼠的肝脏匀浆,棕榈酰辅酶A依赖性NAD⁺还原速率始终低于相应的酰基辅酶A氧化酶活性。这种差异在通过发光法测定的酰基辅酶A氧化酶活性方面最为明显。

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