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Induction and repression of the major phenobarbital-induced cytochrome P-450 measured by radioimmunoassay.

机译:通过放射免疫测定法测定了主要苯巴比妥诱导的细胞色素P-450的诱导和抑制。

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摘要

Two independent radioimmunoassay techniques for the major phenobarbital-inducible cytochrome P-450 (PB P-450) of rat liver microsomal membranes are described. The first technique employs as the source of radiolabelled antigen the products of translation in vitro labelled with [35S]methionine. The second technique employs purified antigen labelled with 125I and is quicker, less expensive and more precise. Both assays are highly specific for PB P-450 and can detect quantities of this variant as small as 1 ng. This is several orders of magnitude more sensitive than any method described previously for the quantification of cytochromes P-450, and consequently the technique is particularly well suited for the quantification of so-called constitutive cytochrome P-450 variants that are present in very low amounts. The results of the radioimmunoassays demonstrate that the apparent 2.6-fold induction of total cytochromes P-450 after phenobarbital treatment is due to a 43-fold increase in Pb P-450. Although beta-naphthoflavone increases the total content of cytochrome P-450 of microsomal membranes 1.4-fold, it actually causes a 55% decrease in the amount of PB P-450. Thus different xenobiotics can have differential effects on the expression of the genes for specific cytochrome P-450 variants.
机译:描述了大鼠肝微粒体膜主要苯巴比妥可诱导的细胞色素P-450(PB P-450)的两种独立的放射免疫分析技术。第一种技术采用体外用[35S]蛋氨酸标记的翻译产物作为放射性标记抗原的来源。第二种技术使用标记有125I的纯化抗原,并且更快,更便宜且更精确。两种测定法对PB P-450都具有高度特异性,并且可以检测到小至1 ng的这种变体。这比以前描述的用于定量细胞色素P-450的任何方法都灵敏几个数量级,因此,该技术特别适合定量含量非常低的所谓组成型细胞色素P-450变体。放射免疫分析的结果表明,苯巴比妥治疗后,总细胞色素P-450的明显2.6倍诱导是由于Pb P-450增加43倍引起的。尽管β-萘黄酮将微粒体膜细胞色素P-450的总含量增加了1.4倍,但实际上导致PB P-450含量降低了55%。因此,不同的异生素可以对特定细胞色素P-450变体的基因表达产生不同的影响。

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