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结核分枝杆菌脂蛋白SodC中O-糖基化位点的N端聚集

N-Terminal clustering of the O-glycosylation sites in the Mycobacterium tuberculosis lipoprotein SodC.

作者信息

Sartain Mark J, Belisle John T

机构信息

Department of Microbiology, Immunology, and Pathology, Mycobacteria Research Laboratories, Colorado State University, Fort Collins, CO 80523, USA.

出版信息

Glycobiology. 2009 Jan;19(1):38-51. doi: 10.1093/glycob/cwn102. Epub 2008 Oct 8.

Abstract

SodC is one of two superoxide dismutases produced by Mycobacterium tuberculosis. This protein was previously shown to contribute to virulence and to act as a B-cell antigen. SodC is also a putative lipoprotein, and like other Sec-translocated mycobacterial proteins it was suggested to be modified with glycosyl units. To definitively define the glycosylation of SodC, we applied an approach that combined site-directed mutagenesis, lectin binding, and mass spectrometry. This resulted in identification of six O-glycosylated residues within a 13-amino-acid region near the N-terminus. Each residue was modified with one to three hexose units, and the most dominant SodC glycoform was modified with nine hexose units. In addition to O-glycosylation of threonine residues, this study provides the first evidence of serine O-glycosylation in mycobacteria. When combined with bioinformatic analyses, the clustering of O-glycosylation appeared to occur in a region of SodC with a disordered structure and not in regions important to the enzymatic activity of SodC. The use of recombinant amino acid substitutions to alter glycosylation sites provided further evidence that glycosylation influences proteolytic processing and ultimately positioning of cell wall proteins.

摘要

SodC是结核分枝杆菌产生的两种超氧化物歧化酶之一。此前已证明该蛋白有助于毒力,并作为B细胞抗原发挥作用。SodC也是一种假定的脂蛋白,与其他通过Sec转运的分枝杆菌蛋白一样,有人认为它会被糖基单元修饰。为了明确界定SodC的糖基化情况,我们采用了一种结合定点诱变、凝集素结合和质谱分析的方法。这使得我们在靠近N端的一个13个氨基酸的区域内鉴定出了6个O-糖基化残基。每个残基被一到三个己糖单元修饰,最主要的SodC糖型被九个己糖单元修饰。除了苏氨酸残基的O-糖基化外,本研究还首次提供了分枝杆菌中丝氨酸O-糖基化的证据。结合生物信息学分析来看,O-糖基化的聚集似乎发生在SodC结构无序的区域,而非对SodC酶活性重要的区域。利用重组氨基酸取代来改变糖基化位点提供了进一步的证据,表明糖基化会影响蛋白水解加工,最终影响细胞壁蛋白的定位。

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