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苦瓜种子核糖核酸酶MC1与2'-UMP或3'-UMP复合的晶体结构揭示了尿苷特异性的结构基础。

Crystal structures of the ribonuclease MC1 from bitter gourd seeds, complexed with 2'-UMP or 3'-UMP, reveal structural basis for uridine specificity.

作者信息

Suzuki A, Yao M, Tanaka I, Numata T, Kikukawa S, Yamasaki N, Kimura M

机构信息

Division of Biological Sciences, Hokkaido University, Sapporo, 060-0810, Japan.

出版信息

Biochem Biophys Res Commun. 2000 Aug 28;275(2):572-6. doi: 10.1006/bbrc.2000.3318.

DOI:10.1006/bbrc.2000.3318
PMID:10964705
Abstract

Ribonuclease MC1 (RNase MC1) isolated from seeds of bitter gourd (Momordica charantia) consists of 190 amino acids and is characterized by a preferential cleavage at the 5'-side of uridine. This uridine specificity distinguishes RNase MC1 from other enzymes belonging to the RNase T2 family. The three-dimensional structures of RNase MC1, in a complex with either 2'-UMP or 3'-UMP, were determined at 1.48 and 1.77 A resolutions, respectively. The side chains of Gln9 and Asn71 interact with O4 and N3, respectively, of the uracil base by hydrogen bondings. In addition, the uracil base is sandwiched by the hydrophobic side chains of Leu73 and Phe80. Compared with these amino acid residues and corresponding residues in RNases in the RNase T2 family, Gln9 and Phe80 are highly conserved in the RNases in T2 family, while Asn71 and Leu73 in RNase MC1 are variant in sequences. It is thus likely that interactions of the side chains of Asn71 and Leu73 with the uracil base are responsible for the absolute uridine specificity of RNase MC1. Site-directed mutagenesis experiments showed that replacement of Asn by Thr decreased both the catalytic efficiency and the binding affinity by 2.3- and 7.0-fold, respectively, and substitution of Leu73 for Ala predominantly decreased the binding affinity by 14. 5-fold, compared with findings in case of wild-type RNase MC1. It is thus demonstrated that Asn71 and Leu73 play an essential role in uridine preference for RNase MC1.

摘要

从苦瓜(Momordica charantia)种子中分离出的核糖核酸酶MC1(RNase MC1)由190个氨基酸组成,其特点是优先在尿苷的5'侧进行切割。这种尿苷特异性使RNase MC1与其他属于RNase T2家族的酶区分开来。分别在1.48 Å和1.77 Å分辨率下测定了与2'-UMP或3'-UMP形成复合物的RNase MC1的三维结构。Gln9和Asn71的侧链分别通过氢键与尿嘧啶碱基的O4和N3相互作用。此外,尿嘧啶碱基被Leu73和Phe80的疏水侧链夹在中间。与RNase T2家族中RNases的这些氨基酸残基和相应残基相比,Gln9和Phe80在T2家族的RNases中高度保守,而RNase MC1中的Asn71和Leu73在序列上是可变的。因此,Asn71和Leu73的侧链与尿嘧啶碱基的相互作用可能是RNase MC1绝对尿苷特异性的原因。定点诱变实验表明,用Thr取代Asn分别使催化效率和结合亲和力降低了2.3倍和7.0倍,与野生型RNase MC1相比,将Leu73替换为Ala主要使结合亲和力降低了14.5倍。因此证明Asn71和Leu73在RNase MC1对尿苷的偏好中起重要作用。

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