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腺病毒2型早期信使核糖核酸中的多个甲基化帽序列。

Multiple methylated cap sequences in adenovirus type 2 early mRNA.

作者信息

Hashimoto S I, Green M

出版信息

J Virol. 1976 Nov;20(2):425-35. doi: 10.1128/JVI.20.2.425-435.1976.

Abstract

The methylated constituents of early adenovirus 2 mRNA were studied. RNA was isolated from polyribosomes of cells double labeled with [methyl-3H]methionine and 32PO4 from 2 to 7 g postinfection in the presence of cycloheximide. Cycloheximide ensures that methylation and processing are performed by preexisting host cell enzymes. RNA was fractionated into polyadenylic [poly(A)]+ and poly(A)- molecules using poly(U)-Sepharose, and undergraded virus-specific RNA was isolated by hybridization to viral DNA in 50% formamide at 37 degrees C. Viral mRNA was digested with RNase T2 and chromatographed on DEAE-Sephadex in 7 M urea. Two 3H-labeled RNase T2-resistant oligonucleotide fractions with charges between -5 and -6 were obtained, consistent with two classes of 5' terminal methyl "cap" structures, m7G(5')ppp(5')NmpNp (cap 1) and m7G(5')ppp(5')NmNmpNp (cap 2) (Nm is a ribose 2'-O-methylation). The putative cap 1 contains all the methylated constituents of cap 1 plus Cm. The molar ratios of m7G to 2'-O-methylnucleosides is about 1.0 for cap 1 and 0.5 for cap 2, consistent with the proposed cap structures. Most significant, compositional analysis indicates four different cap 1 structures and at least three different cap 2 structures. Thus there is a minimum of seven early viral mRNA species with different cap structures, unless each type of mRNA can have more than one 5' terminus. In addition to methylated caps, early mRNA contains internal base methylations, exclusively as m6A, as shown by analyses of the mononucleotide (-2 charge) fraction. m6A was present in the ratio of 1 mol of m6Ap per 450 nucleotides. Thus viral mRNA molecules contain two to three internal m6A residues per methyl cap, since there is on the average 1 cap per 1,250 nucleotides.

摘要

对早期腺病毒2信使核糖核酸(mRNA)的甲基化成分进行了研究。在环己酰亚胺存在的情况下,于感染后2至7小时,从用[甲基-3H]甲硫氨酸和32PO4进行双重标记的细胞的多核糖体中分离出RNA。环己酰亚胺可确保甲基化和加工由预先存在的宿主细胞酶进行。使用聚(U)-琼脂糖凝胶将RNA分离为聚腺苷酸[聚(A)]+和聚(A)-分子,并通过在37℃下于50%甲酰胺中与病毒DNA杂交来分离未分级的病毒特异性RNA。病毒mRNA用核糖核酸酶T2消化,并在含有7M尿素的二乙氨基乙基-琼脂糖凝胶(DEAE-Sephadex)上进行层析。获得了两个3H标记的对核糖核酸酶T2有抗性的寡核苷酸级分,其电荷在-5至-6之间,这与两类5'末端甲基“帽”结构一致,即m7G(5')ppp(5')NmpNp(帽1)和m7G(5')ppp(5')NmNmpNp(帽2)(Nm是核糖2'-O-甲基化)。推测的帽1包含帽1的所有甲基化成分加上Cm。对于帽1,m7G与2'-O-甲基核苷的摩尔比约为1.0,对于帽2为0.5,这与所提出的帽结构一致。最为重要的是,组成分析表明有四种不同的帽1结构和至少三种不同的帽2结构。因此,至少有七种具有不同帽结构的早期病毒mRNA种类,除非每种mRNA类型可以有不止一个5'末端。除了甲基化帽外,早期mRNA还含有内部碱基甲基化,仅为m6A,单核苷酸(-2电荷)级分的分析表明了这一点。m6A的存在比例为每450个核苷酸中有1摩尔m6Ap。因此,病毒mRNA分子每个甲基帽含有两到三个内部m6A残基,因为平均每1250个核苷酸有1个帽。

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