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来自面包酵母和大肠杆菌MRE 600的异亮氨酰-tRNA合成酶。tRNA(Ile)-C-C-A(3'NH2)氨酰化过程中对20种氨基酸的识别

Isoleucyl-tRNA synthetase from baker's yeast and from Escherichia coli MRE 600. Discrimination of 20 amino acids in aminoacylation of tRNA(Ile)-C-C-A(3'NH2).

作者信息

Freist W, Sternbach H, Cramer F

机构信息

Abteilung Chemie, Max-Planck-Institut für Experimentelle Medizin, Göttingen, Federal Republic of Germany.

出版信息

Eur J Biochem. 1987 Nov 16;169(1):33-9. doi: 10.1111/j.1432-1033.1987.tb13577.x.

DOI:10.1111/j.1432-1033.1987.tb13577.x
PMID:3315663
Abstract

For discrimination between isoleucine and the other 19 naturally occurring amino acids by isoleucyl-tRNA synthetases from baker's yeast and from Escherichia coli MRE 600 discrimination factors have been determined from kcat and Km values in aminoacylation of the modified tRNA(Ile)-C-C-A(3'NH2). Discrimination factors D1 are products of an initial discrimination factor and a proof-reading factor: D1 = I1.II1. From discrimination factors and AMP formation stoichiometry factors I1 and II1 were calculated. D1 values obtained with the enzyme from E. coli are generally higher than those observed with the yeast enzyme, in some cases up to ten times. With both enzymes low D1 values are found for cysteine, valine, and tryptophan (20-200), the highest values for glycine, alanine, and serine (600-4000). I1 values calculated for the E. coli enzyme are slightly higher (4-145) than the factors observed with the yeast enzyme (1-85), proof-reading factors II1 of the E. coli enzyme are scattering about a mean value about 70, those of the yeast enzyme about a mean value about 50. Initial discrimination factors I1 are directly related to hydrophobic interaction forces between the substrates and the enzymes. Plots of Gibbs free energy differences calculated from these factors are linearly related to the accessible surface areas of the amino acids. A hypothetical model of the binding site can be given in which selection of amino acids is achieved by hydrophobic forces and removal of steric hindrance.

摘要

为了通过来自面包酵母和大肠杆菌MRE 600的异亮氨酰 - tRNA合成酶区分异亮氨酸与其他19种天然存在的氨基酸,已根据修饰的tRNA(Ile)-C-C-A(3'NH2)氨酰化反应中的kcat和Km值确定了区分因子。区分因子D1是初始区分因子和校对因子的乘积:D1 = I1.II1。根据区分因子和AMP形成化学计量因子计算出I1和II1。用大肠杆菌的酶获得的D1值通常高于用酵母酶观察到的值,在某些情况下高达十倍。对于这两种酶,半胱氨酸、缬氨酸和色氨酸的D1值较低(20 - 200),甘氨酸、丙氨酸和丝氨酸的D1值最高(600 - 4000)。为大肠杆菌的酶计算出的I1值略高于用酵母酶观察到的因子(1 - 85)(4 - 145),大肠杆菌的酶的校对因子II1在平均值约70附近分散,酵母酶的校对因子II1在平均值约50附近分散。初始区分因子I1与底物和酶之间的疏水相互作用力直接相关。根据这些因子计算出的吉布斯自由能差的图与氨基酸的可及表面积呈线性相关。可以给出一个结合位点的假设模型,其中氨基酸的选择是通过疏水力和空间位阻的消除来实现的。

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