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A nested double pseudoknot is required for self-cleavage activity of both the genomic and antigenomic hepatitis delta virus ribozymes.

机译:对于基因组和反基因组肝炎三角洲病毒核酶的自我切割活性需要嵌套的双假结。

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摘要

The crystal structure of a genomic hepatitis delta virus (HDV) ribozyme 3' cleavage product predicts the existence of a 2 bp duplex, P1.1, that had not been previously identified in the HDV ribozymes. P1.1 consists of two canonical C-G base pairs stacked beneath the G.U wobble pair at the cleavage site and would appear to pull together critical structural elements of the ribozyme. P1.1 is the second stem of a second pseudoknot in the ribozyme, making the overall fold of the ribozyme a nested double pseudoknot. Sequence comparison suggests the potential for P1.1 and a similar fold in the antigenomic ribozyme. In this study, the base pairing requirements of P1.1 for cleavage activity were tested in both the genomic and antigenomic HDV ribozymes by mutagenesis. In both sequences, cleavage activity was severely reduced when mismatches were introduced into P1.1, but restored when alternative base pairing combinations were incorporated. Thus, P1.1 is an essential structural element required for cleavage of both the genomic and antigenomic HDV ribozymes and the model for the antigenomic ribozyme secondary structure should also be modified to include P1.1.
机译:基因组乙型肝炎三角洲病毒(HDV)核酶3'裂解产物的晶体结构预测存在2 bp的双链体P1.1,以前在HDV核酶中尚未发现。 P1.1由两个标准的C-G碱基对组成,该碱基对堆叠在裂解位点的G.U摆动对之下,似乎将核酶的关键结构元件拉在一起。 P1.1是核酶中第二个假结的第二个茎,使核酶的整体折叠成为嵌套的双假结。序列比较表明P1.1的潜力和反基因组核酶的相似倍数。在这项研究中,通过诱变在基因组和反基因组HDV核酶中测试了P1.1对切割活性的碱基配对要求。在两个序列中,当错配引入到P1.1中时,切割活性都大大降低,但是当掺入替代的碱基配对组合时,切割活性却恢复了。因此,P1.1是裂解基因组和反基因组HDV核酶所必需的必要结构元件,反基因组核酶二级结构的模型也应修改为包括P1.1。

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