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特定鸟苷N7氮原子和嘌呤氨基对于锤头状核酶高效切割的重要性。

Importance of specific guanosine N7-nitrogens and purine amino groups for efficient cleavage by a hammerhead ribozyme.

作者信息

Fu D J, Rajur S B, McLaughlin L W

机构信息

Department of Chemistry, Boston College, Chestnut Hill, Massachusetts 02167.

出版信息

Biochemistry. 1993 Oct 12;32(40):10629-37. doi: 10.1021/bi00091a013.

DOI:10.1021/bi00091a013
PMID:8399208
Abstract

Seven modified hammerhead ribozyme/substrate complexes have been prepared in which individual purine nitrogens, the guanine N7-, the guanine N2-, or the adenine N6-nitrogen, have been excised. The modified complexes were chemically synthesized with the substitution of a single 7-deazaguanosine (c7G), inosine (I), or nebularine (purine riboside, P) base analogue as appropriate for residues G5, G8, G12, A13, A14, or A15. Two of the base analogues, c7G5 and C7G8, occur in a 19-mer ribozyme, while the remaining three residues are present in a 24-mer substrate. Under stoichiometric conditions, four of the complexes, G5c7G, G8c7G, G12c7G, and A14P, are cleaved with relatively little change in rate when compared with the native complex. Two complexes, A13P and A15P, are cleaved some 6-8-fold slower than the native complex, while the G12I complex is reduced in rate by 50-fold. Steady-state kinetic analyses indicate that the cleavage efficiencies, as measured by kcat/KM values, for the G5c7G, G8c7G, and G12c7G complexes are only marginally reduced relative to the native complex. The values for the A13P, A14P, and A15P complexes are reduced by 25-, 15-, and 60-fold, respectively. These reductions in cleavage efficiency are primarily a result of lower kcat values. By comparison, the kcat/KM value for the G12I complex is decreased 450-fold relative to the native complex and is characterized by an 8-fold increase in KM and a kcat value that is reduced nearly 60-fold. These results indicate that the N2-amino group of G12 in the hammerhead ribozyme/substrate complex is critical for efficient cleavage activity.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

已制备了七种修饰的锤头状核酶/底物复合物,其中单个嘌呤氮原子,即鸟嘌呤的N7-、鸟嘌呤的N2-或腺嘌呤的N6-氮原子已被切除。这些修饰的复合物通过化学合成,用单个7-脱氮鸟苷(c7G)、次黄嘌呤(I)或喷司他丁(嘌呤核糖苷,P)碱基类似物分别取代G5、G8、G12、A13、A14或A15残基。其中两种碱基类似物,c7G5和C7G8,存在于一个19聚体核酶中,而其余三个残基存在于一个24聚体底物中。在化学计量条件下,与天然复合物相比,四种复合物,即G5c7G、G8c7G、G12c7G和A14P,切割时速率变化相对较小。两种复合物,A13P和A15P,则比天然复合物慢约6至8倍,而G12I复合物的速率降低了50倍。稳态动力学分析表明,通过kcat/KM值衡量,G5c7G、G8c7G和G12c7G复合物的切割效率相对于天然复合物仅略有降低。A13P、A14P和A15P复合物的值分别降低了25倍、15倍和60倍。这些切割效率的降低主要是由于kcat值较低。相比之下,G12I复合物的kcat/KM值相对于天然复合物降低了450倍,其特征是KM增加了8倍,kcat值降低了近60倍。这些结果表明,锤头状核酶/底物复合物中G12的N2-氨基对于有效的切割活性至关重要。(摘要截断于250字)

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