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A continuous kinetic assay for RNA-cleaving deoxyribozymes, exploiting ethidium bromide as an extrinsic fluorescent probe

机译:利用溴化乙锭作为外在荧光探针进行RNA裂解脱氧核酶的连续动力学测定

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摘要

We describe a rapid and inexpensive method to monitor the kinetics of small RNA-cleaving deoxyribozymes, based on the exogenous fluorophore ethidium bromide. Ethidium binds preferentially to double-stranded nucleic acids, and its fluorescence emission increases dramatically upon intercalation. Thus, ethidium can be used in single-turnover experiments to measure both annealing of the deoxyribozyme to its substrate and release of the products. Under conditions in which dissociation of the product is fast compared with cleavage, the apparent rate of product release reflects the cleavage step. The method was developed for characterizing the so-called 8-17 catalytic DNA, but its general applicability in the deoxyribozyme field was verified using the 10-23 RNA-cleaving construct. Catalysis by both deoxyribozymes was not inhibited in the presence of substoichiometric amounts of ethidium, and the rates obtained through the ethidium assay were virtually identical to the rates determined using radiolabeled substrates. In contrast, the assay cannot be applied to the large, structured ribozymes, and its use to study the kinetics of the small hammerhead ribozyme was hampered by the presence on the catalyst of at least one high-affinity ethidium binding site.
机译:我们描述了一种基于外源荧光团溴化乙锭监测小RNA裂解脱氧核酶的动力学的快速而廉价的方法。乙硫醇优先与双链核酸结合,插入时其荧光发射显着增加。因此,可将乙锭用于单周转实验中,以测量脱氧核糖酶向其底物的退火和产物的释放。在产物的解离与解离相比快速解离的条件下,表观的产物释放速率反映了解离步骤。已开发出该方法用于表征所谓的8-17催化DNA,但是使用10-23 RNA切割构建体验证了其在脱氧核酶领域的普遍适用性。在亚化学计量的乙锭存在下,两种脱氧核酶的催化作用均未受到抑制,通过乙锭测定获得的速率实际上与使用放射性标记底物测定的速率相同。相反,该测定法不能应用于大的结构化核酶,并且其用于研究小锤头状核酶的动力学的方法由于在催化剂上存在至少一个高亲和力乙锭结合位点而受到阻碍。

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