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Partial purification of a 6-methyladenine mRNA methyltransferase which modifies internal adenine residues.

机译:部分纯化6-甲基腺嘌呤mRNA甲基转移酶可修饰内部腺嘌呤残基。

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摘要

Two forms of a 6-methyladenine mRNA methyltransferase have been partially purified using a T7 transcript coding for mouse dihydrofolate reductase as an RNA substrate. Both enzyme forms modify internal adenine residues within the RNA substrate. The enzymes were purified 357- and 37-fold respectively from nuclear salt extracts prepared from HeLa cells using DEAE-cellulose and phosphocellulose chromatography. The activity of the first form of the enzyme eluted from DEAE-cellulose (major form) was at least 3-fold greater than that of the second (minor form). H.p.l.c. analysis of the hydrolysed, methylated mRNA substrates demonstrated that both forms of the enzyme produced only 6-methyladenine. The two forms of the enzyme differed in their RNA substrate specificity as well as in the dependence for a 5' cap structure. The 6-methyladenine mRNA methyltransferase activity was found to be elevated in HeLa nuclei as compared with nuclear extracts from rat kidney and brain. Enzymic activity could not be detected in nuclei from either normal rat liver or regenerating rat liver. In the case of the HeLa cell, activity could only be detected in nuclear extracts, with a small amount in the ribosomal fraction. Other HeLa subcellular fractions were void of activity.
机译:两种形式的6-甲基腺嘌呤mRNA甲基转移酶已使用编码小鼠二氢叶酸还原酶作为RNA底物的T7转录本进行了部分纯化。两种酶形式均修饰RNA底物内的内部腺嘌呤残基。使用DEAE-纤维素和磷酸纤维素色谱法分别从HeLa细胞制备的核盐提取物中将酶纯化了357倍和37倍。从DEAE纤维素(主要形式)洗脱的酶的第一种形式的活性至少是第二种(次要形式)的活性的3倍。 H.p.l.c.水解的甲基化mRNA底物的分析表明,两种形式的酶仅产生6-甲基腺嘌呤。两种形式的酶的RNA底物特异性以及对5'帽结构的依赖性不同。与来自大鼠肾脏和大脑的核提取物相比,在HeLa核中发现了6-甲基腺嘌呤mRNA甲基转移酶活性升高。在正常大鼠肝脏或再生大鼠肝脏的细胞核中均未检测到酶活性。在HeLa细胞的情况下,只能在核提取物中检测到活性,而核糖体组分中的含量很少。其他HeLa亚细胞级分没有活性。

著录项

  • 期刊名称 Biochemical Journal
  • 作者

    M T Tuck;

  • 作者单位
  • 年(卷),期 1992(288),Pt 1
  • 年度 1992
  • 页码 233–240
  • 总页数 8
  • 原文格式 PDF
  • 正文语种
  • 中图分类 分子生物学;
  • 关键词

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