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色氨酸59被酪氨酸取代增强了核糖核酸酶T1以及24、42和45位酪氨酸到色氨酸变体的催化活性。

Trp59 to Tyr substitution enhances the catalytic activity of RNase T1 and of the Tyr to Trp variants in positions 24, 42 and 45.

作者信息

Grunert H P, Landt O, Zirpel-Giesebrecht M, Backmann J, Heinemann U, Saenger W, Hahn U

机构信息

Institut für Biochemie, Medizinische Universität zu Lübeck, Germany.

出版信息

Protein Eng. 1993 Sep;6(7):739-44. doi: 10.1093/protein/6.7.739.

DOI:10.1093/protein/6.7.739
PMID:8248097
Abstract

Using point mutated overproducing strains of E. coli, ribonuclease T1 was prepared with the single substitutions Tyr24Trp, Tyr42Trp, Tyr45Trp or Trp59Tyr and the corresponding double substitutions Tyr24Trp/Trp59Tyr, Tyr42Trp/Trp59Tyr and Tyr45Trp/Trp59Tyr. Steady state kinetics of the transesterification reaction for the two dinucleoside monophosphate substrates guanylyl-3',5'-cytidine and guanylyl-3',5'-adenosine indicate that the tryptophan can be introduced in different positions within the ribonuclease T1 molecule without abolishing enzymatic activity. The Trp59Tyr exchange even enhances catalysis of the cleavage reaction (kcat/Km) relative to the wild type enzyme and similar effects are found with single tyrosine to tryptophan substitutions. For the pH dependencies of the guanylyl-3',5'-cytidine transesterification reaction of wild type ribonuclease T1 and of the variants, typically bell-shaped curves are observed with a plateau in the range pH 4.5-7.0. Their shapes and slopes indicate that the enzymes are comparable in their macroscopic pKa values. At pH 7.5, the variant Tyr45Trp/Trp59Tyr shows a more than 3-fold higher transesterification activity for guanylyl-3',5'-adenosine and a 2-fold increase for guanylyl-3',5'-cytidine compared to the wild type enzyme, i.e. this variant catalyses the transesterification of the substrate guanylyl-3',5'-adenosine with the same or better efficiency as guanylyl-3',5'-cytidine.

摘要

利用大肠杆菌的点突变高产菌株,制备了核糖核酸酶T1的单取代突变体Tyr24Trp、Tyr42Trp、Tyr45Trp或Trp59Tyr,以及相应的双取代突变体Tyr24Trp/Trp59Tyr、Tyr42Trp/Trp59Tyr和Tyr45Trp/Trp59Tyr。对于两种二核苷单磷酸底物鸟苷酰-3',5'-胞苷和鸟苷酰-3',5'-腺苷的酯交换反应的稳态动力学表明,色氨酸可以引入核糖核酸酶T1分子内的不同位置而不丧失酶活性。相对于野生型酶,Trp59Tyr交换甚至增强了切割反应的催化作用(kcat/Km),并且在单个酪氨酸到色氨酸的取代中也发现了类似的效果。对于野生型核糖核酸酶T1及其变体的鸟苷酰-3',5'-胞苷酯交换反应的pH依赖性,通常观察到钟形曲线,在pH 4.5-7.0范围内有一个平稳期。它们的形状和斜率表明这些酶在宏观pKa值方面具有可比性。在pH 7.5时,与野生型酶相比,变体Tyr45Trp/Trp59Tyr对鸟苷酰-3',5'-腺苷的酯交换活性高出3倍以上,对鸟苷酰-3',5'-胞苷的酯交换活性提高了2倍,即该变体催化底物鸟苷酰-3',5'-腺苷的酯交换反应的效率与鸟苷酰-3',5'-胞苷相同或更高。

相似文献

1
Trp59 to Tyr substitution enhances the catalytic activity of RNase T1 and of the Tyr to Trp variants in positions 24, 42 and 45.色氨酸59被酪氨酸取代增强了核糖核酸酶T1以及24、42和45位酪氨酸到色氨酸变体的催化活性。
Protein Eng. 1993 Sep;6(7):739-44. doi: 10.1093/protein/6.7.739.
2
RNase T1 variant RV cleaves single-stranded RNA after purines due to specific recognition by the Asn46 side chain amide.核糖核酸酶T1变体RV由于天冬酰胺46侧链酰胺的特异性识别,在嘌呤之后切割单链RNA。
Biochemistry. 2004 Mar 16;43(10):2854-62. doi: 10.1021/bi035961f.
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Modification of ribonuclease T1 specificity by random mutagenesis of the substrate binding segment.通过对底物结合片段进行随机诱变来改变核糖核酸酶T1的特异性。
Biochemistry. 1999 Jan 26;38(4):1371-6. doi: 10.1021/bi9817515.
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Subsite interactions of ribonuclease T1: viscosity effects indicate that the rate-limiting step of GpN transesterification depends on the nature of N.核糖核酸酶T1的亚位点相互作用:粘度效应表明GpN酯交换反应的限速步骤取决于N的性质。
Biochemistry. 1991 Sep 3;30(35):8661-5. doi: 10.1021/bi00099a024.
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X-ray crystallographic and calorimetric studies of the effects of the mutation Trp59-->Tyr in ribonuclease T1.
Eur J Biochem. 1994 Mar 1;220(2):527-34. doi: 10.1111/j.1432-1033.1994.tb18652.x.
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Crystal structure of the Tyr45Trp mutant of ribonuclease T1 in a complex with 2'-adenylic acid.
Eur J Biochem. 1991 Oct 1;201(1):199-202. doi: 10.1111/j.1432-1033.1991.tb16274.x.
7
Purine activity of RNase T1RV is further improved by substitution of Trp59 by tyrosine.通过用酪氨酸取代色氨酸59,核糖核酸酶T1RV的嘌呤活性进一步提高。
Biochem Biophys Res Commun. 2005 Oct 28;336(3):882-9. doi: 10.1016/j.bbrc.2005.08.188.
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Kinetic studies of guanine recognition and a phosphate group subsite on ribonuclease T1 using substitution mutants at Glu46 and Lys41.利用核糖核酸酶T1上Glu46和Lys41位点的取代突变体对鸟嘌呤识别及磷酸基团亚位点进行动力学研究。
Arch Biochem Biophys. 2002 Oct 1;406(1):73-7. doi: 10.1016/s0003-9861(02)00409-5.
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Probing functional perfection in substructures of ribonuclease T1: double combinatorial random mutagenesis involving Asn43, Asn44, and Glu46 in the guanine binding loop.探究核糖核酸酶T1亚结构中的功能完善:涉及鸟嘌呤结合环中Asn43、Asn44和Glu46的双重组合随机诱变
Biochemistry. 2001 Mar 27;40(12):3748-57. doi: 10.1021/bi002837c.
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Ribonuclease T1 is active when both catalytic histidines are replaced by aspartate.当两个催化性组氨酸被天冬氨酸取代时,核糖核酸酶T1仍具有活性。
Biol Chem. 1997 Jun;378(6):553-8. doi: 10.1515/bchm.1997.378.6.553.

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