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[MS2噬菌体RNA复制酶顺反子的调控区。MS2 RNA特异性片段对T1核糖核酸酶消化及用乙二醛进行化学修饰的可及性]

[Regulatory region of the MS2 phage RNA replicase cistron. Accesibility of MS2 RNA specific fragment to T1 RNAse digestion and chemical modification with kethoxal].

作者信息

Berzin' V M, Iansone I V, Gribanov V A, Tsimanis A Iu, Gren E Ia

出版信息

Mol Biol (Mosk). 1978 Nov-Dec;12(6):1288-98.

PMID:106237
Abstract

Partial digestion with T1 RNAase and chemical modification with kethoxal were used to study stability of two hairpin in the proposed secondary structure of the functionally active MS2 RNA fragment MS2 R(--53 leads to 6), containing the regulatory region of the phage replicase cistron. Analysis of the products obtained after the above treatments showed that T1 RNAase and kethoxal attacked predominantly the guanosine residues in the hairpin b of the MS2 R(--53 leads to 6). This implies that in contrast to the structurally stable hairpin a of the polynucleotide, hairpin b appears to be more labile and may exist under the present experimental conditions in equilibrium with its open form. The data of the competition experiments demonstrated that the kethoxal modified MS2 R(-53 leads to 6) and shorter polynucleotide MS2 R(-53 leads to-11) obtained from MS2 R(-53 leads to 6) after T1 RNAase digestion failed to bind with MS2 coat protein. The relatively unstable hairpin b region in the polynucleotide MS2 R(-53 leads to 6) is suggested to play essential role in the complex formation.

摘要

使用T1核糖核酸酶进行部分消化以及用乙二醛进行化学修饰,以研究功能活性MS2 RNA片段MS2 R(-53至6)的二级结构中两个发夹结构的稳定性,该片段包含噬菌体复制酶顺反子的调控区域。对上述处理后获得的产物进行分析表明,T1核糖核酸酶和乙二醛主要攻击MS2 R(-53至6)发夹b中的鸟苷残基。这意味着,与多核苷酸结构稳定的发夹a相比,发夹b似乎更不稳定,并且在当前实验条件下可能与其开放形式处于平衡状态。竞争实验的数据表明,乙二醛修饰的MS2 R(-53至6)以及T1核糖核酸酶消化后从MS2 R(-53至6)获得的较短多核苷酸MS2 R(-53至-11)无法与MS2外壳蛋白结合。多核苷酸MS2 R(-53至6)中相对不稳定的发夹b区域被认为在复合物形成中起重要作用。

相似文献

1
[Regulatory region of the MS2 phage RNA replicase cistron. Accesibility of MS2 RNA specific fragment to T1 RNAse digestion and chemical modification with kethoxal].[MS2噬菌体RNA复制酶顺反子的调控区。MS2 RNA特异性片段对T1核糖核酸酶消化及用乙二醛进行化学修饰的可及性]
Mol Biol (Mosk). 1978 Nov-Dec;12(6):1288-98.
2
The regulatory region of MS2 phage RNA replicase cistron. III. Characterization of fragments resulting from S1 nuclease digestion.MS2噬菌体RNA复制酶顺反子的调控区域。III. S1核酸酶消化产生的片段的特性分析。
Nucleic Acids Res. 1979;6(5):1747-60. doi: 10.1093/nar/6.5.1747.
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Secondary structure of the 5' end of bacteriophage MS2 RNA Methoxyamine and kethoxal modification.噬菌体MS2 RNA 5'端的二级结构:甲氧基胺和乙二醛修饰
Eur J Biochem. 1979 Dec 17;102(2):595-604. doi: 10.1111/j.1432-1033.1979.tb04277.x.
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[Regulatory region of fr phage replicase cistron. II. Isolation and structure of specific fr RNA fragments].[噬菌体复制酶顺反子的调控区。II. 特异性fr RNA片段的分离与结构]
Mol Biol (Mosk). 1982 Sep-Oct;16(5):1109-15.
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The regulatory region of MS2 phage RNA replicase cistron. IV. Functional activity of specific MS2 RNA fragments in formation of the 70 S initiation complex of protein biosynthesis.MS2噬菌体RNA复制酶顺反子的调控区。IV. 特定MS2 RNA片段在蛋白质生物合成70S起始复合物形成中的功能活性。
Nucleic Acids Res. 1979;6(5):1761-74. doi: 10.1093/nar/6.5.1761.
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[Regulatory region of the cistron of phage MS2 RNA replicase. Isolation and characteristics of specific RNA fragments].[噬菌体MS2 RNA复制酶顺反子的调控区。特定RNA片段的分离与特性]
Dokl Akad Nauk SSSR. 1976;229(3):741-4.
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[Ribosomal protein S1 in the complex of E. coli ribosomal subunit 30S with phage MS2 RNA interacts with internal region of the replicase gene].[大肠杆菌核糖体30S亚基与噬菌体MS2 RNA复合物中的核糖体蛋白S1与复制酶基因内部区域相互作用]
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Sequence determination of Gp-rich oligonucleotides by means of the Kethoxal modification.
FEBS Lett. 1976 Jul 1;66(1):77-81. doi: 10.1016/0014-5793(76)80589-3.
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[The ratio of coat protein to bacteriophage f2 RNA in the translational repressor complex].[翻译阻遏复合物中衣壳蛋白与噬菌体f2 RNA的比例]
Mol Biol (Mosk). 1975 Jan-Feb;9(1):78-85.
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Crystal structure of an RNA bacteriophage coat protein-operator complex.一种RNA噬菌体外壳蛋白-操纵基因复合物的晶体结构。
Nature. 1994 Oct 13;371(6498):623-6. doi: 10.1038/371623a0.

引用本文的文献

1
The regulatory region of MS2 phage RNA replicase cistron. III. Characterization of fragments resulting from S1 nuclease digestion.MS2噬菌体RNA复制酶顺反子的调控区域。III. S1核酸酶消化产生的片段的特性分析。
Nucleic Acids Res. 1979;6(5):1747-60. doi: 10.1093/nar/6.5.1747.