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在药物诱导条件下,利用克隆DNA的特异性探针滴定大鼠肝脏中细胞色素P - 450c和P - 450d的mRNA。

Titration of mRNAs for cytochrome P-450c and P-450d under drug-inductive conditions in rat livers by their specific probes of cloned DNAs.

作者信息

Kawajiri K, Gotoh O, Tagashira Y, Sogawa K, Fujii-Kuriyama Y

出版信息

J Biol Chem. 1984 Aug 25;259(16):10145-9.

PMID:6547950
Abstract

By sequence analysis of the cloned cDNA or genomic DNA, we have recently deduced the complete primary structures of two forms of 3-methylcholanthrene-inducible cytochromes P-450 (P-450c and P-450d). Comparing these sequences, we identified two highly conserved regions, amino acid numbers from 35 to 200 and from 340 to 470. The nucleotide sequences corresponding to these homologous regions are also well conserved, whereas other regions have undergone considerable sequence divergence. In RNA blot analysis with unfractionated mRNA isolated from 3-methylcholanthrene-treated rat livers, Probe A (specific to P-450c sequence) hybridized with mRNA around 23 S, while Probe B (specific to P-450d sequence) hybridized with mRNA around 18 S. When common sequence between P-450c and P-450d was used as the probes (Probe C or D), two bands were clearly observed around 23 and 18 S mRNAs. With the common DNA sequence between P-450c and P-450d as a probe (93.7% homology), we studied the induction of specific mRNA for P-450c and P-450d by a single dose of several chemical compounds to rats. 3-Methylcholanthrene increased both P-450c and P-450d mRNA levels by 50 and 10 times above the control at 17 h after the administration, respectively. Despite the lower induction rates, the P-450d mRNA level was constantly higher than or at least similar to that of P-450c mRNA. beta-Naphthoflavone and Kaneclor KC 500 showed similar induction ability to 3-methylcholanthrene. On the other hand, isosafrole induced P-450d mRNA to a much greater extent than P-450c mRNA.

摘要

通过对克隆的互补DNA(cDNA)或基因组DNA进行序列分析,我们最近推导了两种形式的3-甲基胆蒽诱导型细胞色素P-450(P-450c和P-450d)的完整一级结构。比较这些序列时,我们确定了两个高度保守的区域,氨基酸编号分别为35至200以及340至470。与这些同源区域相对应的核苷酸序列也高度保守,而其他区域则经历了相当大的序列分歧。在用从3-甲基胆蒽处理的大鼠肝脏中分离出的未分级信使核糖核酸(mRNA)进行的RNA印迹分析中,探针A(对P-450c序列特异)与约23S的mRNA杂交,而探针B(对P-450d序列特异)与约18S的mRNA杂交。当使用P-450c和P-450d之间的共同序列作为探针(探针C或D)时,在23S和18S mRNA附近清楚地观察到两条带。以P-450c和P-450d之间的共同DNA序列作为探针(同源性为93.7%),我们研究了几种化合物单剂量给药对大鼠后P-450c和P-450d特异性mRNA的诱导情况。给药后17小时,3-甲基胆蒽使P-450c和P-450d的mRNA水平分别比对照增加50倍和10倍。尽管诱导率较低,但P-450d的mRNA水平始终高于或至少与P-450c的mRNA水平相似。β-萘黄酮和氯丹KC 500显示出与3-甲基胆蒽相似的诱导能力。另一方面,异黄樟素诱导P-450d的mRNA的程度比诱导P-450c的mRNA的程度大得多。

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