Bhat B M, Wold W S
Mol Cell Biol. 1985 Nov;5(11):3183-93. doi: 10.1128/mcb.5.11.3183-3193.1985.
We mapped the location of the E3A RNA 3' end site in the E3 transcription unit of adenovirus 2. The procedure used was nuclease-gel analysis with 32P-labeled RNA probes. The poly(A) addition sites were microheterogeneous and were located approximately 17 to 29 nucleotides downstream from an ATTAAA sequence. To identify the sequences that make up the E3A RNA 3' end signal, we constructed five viable virus mutants with deletions in or near the E3A RNA 3' end site. The mutants were analyzed for E3A RNA 3' end formation in vivo. No effect was observed from a 47-base-pair (bp) deletion (dl716) or a 72-bp deletion (dl714) located 22 and 19 nucleotides, respectively, upstream of the ATTAAA. In contrast, E3A RNA 3' end formation was abolished by a 554-bp deletion (dl708) that removes both the ATTAAA and the poly(A) addition sites, a 124-bp deletion (dl713) that removes the ATTAAA but leaves the poly(A) addition sites, and a 65-bp deletion (dl719) that leaves the ATTAAA but removes the poly(A) addition sites. These results indicate that the ATTAAA, as well as downstream sequences, including the poly(A) addition sites, are required for E3A RNA 3' end formation.
我们绘制了腺病毒2型E3转录单元中E3A RNA 3'末端位点的位置。所采用的方法是用32P标记的RNA探针进行核酸酶凝胶分析。聚腺苷酸(poly(A))添加位点存在微异质性,位于ATTAAA序列下游约17至29个核苷酸处。为了鉴定构成E3A RNA 3'末端信号的序列,我们构建了五个在E3A RNA 3'末端位点或其附近有缺失的可行病毒突变体。对这些突变体进行了体内E3A RNA 3'末端形成的分析。在ATTAAA上游分别位于22和19个核苷酸处的47个碱基对(bp)缺失(dl716)或72 bp缺失(dl714)未观察到影响。相反,E3A RNA 3'末端形成被一个554 bp缺失(dl708)消除,该缺失去除了ATTAAA和聚腺苷酸添加位点;一个124 bp缺失(dl713),该缺失去除了ATTAAA但保留了聚腺苷酸添加位点;以及一个65 bp缺失(dl719),该缺失保留了ATTAAA但去除了聚腺苷酸添加位点。这些结果表明,ATTAAA以及包括聚腺苷酸添加位点在内的下游序列是E3A RNA 3'末端形成所必需的。
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