首页> 美国卫生研究院文献>Biochemical Journal >Immunochemical studies of haem oxygenase. Preparation and characterization of antibodies to chick liver haem oxygenase and their use in detecting and quantifying amounts of haem oxygenase protein.
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Immunochemical studies of haem oxygenase. Preparation and characterization of antibodies to chick liver haem oxygenase and their use in detecting and quantifying amounts of haem oxygenase protein.

机译:血红素加氧酶的免疫化学研究。鸡肝血红素加氧酶抗体的制备表征及其在检测和定量血红素加氧酶蛋白中的应用。

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摘要

Monospecific polyclonal rabbit antibodies to a purified form of haem oxygenase of chick liver, showing sequence similarity to mammalian haem oxygenase-1, were raised and used to study characteristics of the oxygenase. The antibodies inhibited activity of the purified oxygenase, but not other enzyme components (NADPH:cytochrome reductase and biliverdin reductase) of the standard assay mixture of haem oxygenase. In addition, the antibodies inhibited activity of haem oxygenase in microsomes (microsomal fractions) from Cd(2+)-treated chick liver, spleen, testis and brain. Western (immuno-) blots of microsomal proteins of selected organs from chick, rat and man, and homogenates of chick-embryo liver-cell cultures, probed with the antibodies, showed a major protein with a molecular mass of 33-34 kDa and a lower-molecular-mass protein (28-29 kDa) of variable intensity. Studies with trypsin and selected proteinase inhibitors established that the smaller peptide was a proteolytic product of the larger. Treatment of chick-embryo liver-cell cultures with CdCl2, a potent inducer of haem oxygenase, increased the degree of proteinase-mediated cleavage of the 33 kDa protein to the lower-molecular-mass form. These results indicate that, under at least some conditions, such cultures should be homogenized in the presence of trypsin inhibitor to prevent proteolytic degradation of the enzyme and allow maximal expression of haem oxygenase activity. The antibodies also reacted with haem oxygenase from spleen, testis and brain of both chicks and rats, and the spleen of humans. A method for quantifying the amount of haem oxygenase protein was developed with use of slot-blots and laser densitometry; linearity was observed from 0 to 5 ng of haem oxygenase protein per slot, and the method was applied to sonicated cultured chick-embryo liver cells treated with Cd2+ (0.3 mM) or iron plus glutethimide. In both cases, increases in enzyme activity were of similar magnitude to increases in amounts of enzyme protein. Approximate amounts of haem oxygenase protein in microsomes of several organs from intact animals could also be estimated by the use of slot-blot-laser densitometry, and the amounts measured were increased by the addition of purified haem oxygenase to the microsomal preparations. Results of these studies indicated that haem oxygenase-1 could be detected in microsomes from all chick or rat organs studied, including testis and brain.(ABSTRACT TRUNCATED AT 400 WORDS)
机译:产生了与哺乳动物血红素加氧酶-1序列相似的纯化形式的鸡肝血红素加氧酶的单特异性多克隆兔抗体,并用于研究该加氧酶的特性。抗体抑制纯化的加氧酶的活性,但抑制血红素加氧酶标准测定混合物中的其他酶成分(NADPH:细胞色素还原酶和胆绿素还原酶)。此外,该抗体抑制了Cd(2+)处理的鸡肝,脾脏,睾丸和脑中微粒体(微粒体级分)中血红素氧化酶的活性。用抗体探测的,来自鸡,大鼠和人的选定器官的微粒体蛋白以及鸡胚肝细胞培养物匀浆的蛋白质(免疫)印迹显示分子量为33-34 kDa的主要蛋白强度可变的低分子质量蛋白质(28-29 kDa)。用胰蛋白酶和选定的蛋白酶抑制剂进行的研究确定较小的肽是较大的肽的蛋白水解产物。用血红素加氧酶的强效诱导剂CdCl2处理鸡胚肝细胞培养物,可将蛋白酶介导的33 kDa蛋白的裂解程度提高为低分子质量形式。这些结果表明,在至少某些条件下,应在胰蛋白酶抑制剂的存在下匀浆此类培养物,以防止酶的蛋白水解降解并允许血红素加氧酶活性的最大表达。抗体还与小鸡​​和大鼠的脾脏,睾丸和大脑以及人的脾脏中的血红素加氧酶反应。利用狭缝印迹和激光光密度法开发了一种定量血红素氧化酶蛋白含量的方法。从每个插槽0到5 ng血红素加氧酶蛋白观察到线性,并将该方法应用于经超声处理的Cd2 +(0.3 mM)或铁加谷氨酰胺处理的鸡胚肝细胞。在这两种情况下,酶活性的增加与酶蛋白量的增加具有相似的幅度。完整动物几个器官微粒体中的血红素加氧酶蛋白的大约量也可以通过缝隙-激光-激光光密度法进行估算,并且通过向微粒体制剂中添加纯化的血红素加氧酶来增加测定的量。这些研究结果表明,在所有研究的小鸡或大鼠器官,包括睾丸和脑中,微粒体中都可以检测到血红素加氧酶-1。(摘要截短了400字)

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