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糖结合活性的烟草凝集素突变分析。

Mutational analysis of the carbohydrate binding activity of the tobacco lectin.

机构信息

Department of Molecular Biotechnology, Laboratory of Biochemistry and Glycobiology, Ghent University, Coupure Links 653, 9000 Ghent, Belgium.

出版信息

Glycoconj J. 2010 Aug;27(6):613-23. doi: 10.1007/s10719-010-9305-2. Epub 2010 Aug 19.

Abstract

At present the three-dimensional structure of the tobacco lectin, further referred to as Nictaba, and its carbohydrate-binding site are unresolved. In this paper, we propose a three-dimensional model for the Nictaba domain based on the homology between Nictaba and the carbohydrate-binding module 22 of Clostridium thermocellum Xyn10B. The suggested model nicely fits with results from circular dichroism experiments, indicating that Nictaba consists mainly of β-sheet. In addition, the previously identified nuclear localization signal is located at the top of the protein as a part of a protruding loop. Judging from this model and sequence alignments with closely related proteins, conserved glutamic acid and tryptophan residues in the Nictaba sequence were selected for mutational analysis. The mutant DNA sequences as well as the original Nictaba sequence have been expressed in Pichia pastoris and the recombinant proteins were purified from the culture medium. Subsequently, the recombinant proteins were characterized and their carbohydrate binding properties analyzed with glycan array technology. It was shown that mutation of glutamic acid residues in the C-terminal half of the protein did not alter the carbohydrate-binding activity of the lectin. In contrast, mutation of tryptophan residues in the N-terminal half of the Nictaba domain resulted in a complete loss of carbohydrate binding activity. These results suggest that tryptophan residues play an important role in the carbohydrate binding site of Nictaba.

摘要

目前,烟草凝集素(也称为 Nictaba)的三维结构及其碳水化合物结合位点尚未得到解决。本文基于 Nictaba 与热纤梭菌内切木聚糖酶 Xyn10B 的碳水化合物结合模块 22 之间的同源性,提出了一个 Nictaba 结构域的三维模型。该模型与圆二色性实验结果非常吻合,表明 Nictaba 主要由β-折叠组成。此外,先前鉴定的核定位信号位于蛋白质的顶部,作为突出环的一部分。从这个模型和与密切相关的蛋白质的序列比对来看,在 Nictaba 序列中选择了保守的谷氨酸和色氨酸残基进行突变分析。突变后的 DNA 序列以及原始的 Nictaba 序列已在毕赤酵母中表达,并从培养基中纯化了重组蛋白。随后,利用聚糖阵列技术对重组蛋白进行了表征,并分析了其碳水化合物结合特性。结果表明,突变蛋白 C 末端半胱氨酸残基中的谷氨酸残基不会改变凝集素的碳水化合物结合活性。相比之下,突变 Nictaba 结构域 N 端色氨酸残基会导致碳水化合物结合活性完全丧失。这些结果表明,色氨酸残基在 Nictaba 的碳水化合物结合位点中起着重要作用。

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