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基于寡核苷酸的人工核酸酶(OBAN)系统。RNA凸起切割中凸起大小依赖性及催化基团的定位。

Oligonucleotide based artificial nuclease (OBAN) systems. Bulge size dependence and positioning of catalytic group in cleavage of RNA-bulges.

作者信息

Aström Hans, Williams Nicholas H, Strömberg Roger

机构信息

Division of Organic and Bioorganic Chemistry, MBB, Scheele Laboratory, Karolinska Institutet, S-17177 Stockholm, Sweden.

出版信息

Org Biomol Chem. 2003 May 7;1(9):1461-5. doi: 10.1039/b212216b.

DOI:10.1039/b212216b
PMID:12926273
Abstract

Three zinc ion dependent oligonucleotide based artificial nucleases (OBANs) have been synthesized. These consist of 2'-O-methyloligoribonucleosides connected to 5-amino-2,9-dimethylphenanthroline via a urea function to a linker extending either from C-5 of deoxyuridine or from the 2'-position of uridine moieties. Both types of linkers are placed centrally in the modified sequence and in addition one OBAN carries the C-5 modified dU as an additional nucleoside unit at the 5'-end. All three OBANs are shown to cleave target oligoribonucleotides selectively. The target RNA's are varied to form differently sized bulges (0-5 nucleotides (nt)) and the different OBANs have different preferences for which sizes are preferentially cleaved. The OBAN with the centrally positioned C-5 linked zinc chelate preferentially cleaves 3 and 4-nt bulges, the OBAN with the 2'-linked chelate has a preference for slightly smaller bulges and the OBAN with a 5'-end chelate is more efficient the larger the bulge is. In addition the OBAN with the centrally positioned C-5 linked zinc chelate is shown to be a real enzyme, capable of turnover of substrate and displaying Michaelis-Menten behaviour. The main differences in efficiency of cleavage between the different OBAN-RNA substrate combinations are likely to be due to proximity factors i.e. the positioning of a catalytic group relative to cleaved phosphodiester functions. The model systems investigated partially display the importance of catalytic group positioning and should be useful in future development of more efficient OBANs.

摘要

已经合成了三种基于锌离子的寡核苷酸人工核酸酶(OBANs)。它们由通过脲功能连接到5-氨基-2,9-二甲基菲咯啉的2'-O-甲基寡核糖核苷组成,该脲功能连接到从脱氧尿苷的C-5或尿苷部分的2'-位置延伸的接头。两种类型的接头都位于修饰序列的中心,此外,一种OBAN在5'-末端携带C-5修饰的dU作为额外的核苷单元。所有三种OBANs都显示出能选择性地切割靶寡核糖核苷酸。靶RNA被改变以形成不同大小的凸起(0-5个核苷酸(nt)),不同的OBANs对优先切割的大小有不同的偏好。具有中心位置C-5连接锌螯合物的OBAN优先切割3和4-nt的凸起,具有2'-连接螯合物的OBAN偏好稍小的凸起,而具有5'-末端螯合物的OBAN在凸起越大时效率越高。此外,具有中心位置C-5连接锌螯合物的OBAN被证明是一种真正的酶,能够使底物周转并表现出米氏行为。不同OBAN-RNA底物组合之间切割效率的主要差异可能是由于邻近因素,即催化基团相对于切割的磷酸二酯功能的定位。所研究的模型系统部分显示了催化基团定位的重要性,并且应该对未来更高效的OBANs的开发有用。

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