Tullius Michael V, Phillips Nancy J, Scheffler N Karoline, Samuels Nicole M, Munson Jr Robert S, Hansen Eric J, Stevens-Riley Marla, Campagnari Anthony A, Gibson Bradford W
Department of Pharmaceutical Chemistry, University of California, San Francisco, California 94143-0446, USA.
Infect Immun. 2002 Jun;70(6):2853-61. doi: 10.1128/IAI.70.6.2853-2861.2002.
All Haemophilus ducreyi strains examined contain a lipooligosaccharide (LOS) consisting of a single but variable branch oligosaccharide that emanates off the first heptose (Hep-I) of a conserved Hep(3)-phosphorylated 3-deoxy-D-manno-octulosonic acid-lipid A core. In a previous report, identification of tandem genes, lbgA and lbgB, that are involved in LOS biosynthesis was described (Stevens et al., Infect. Immun. 65:651-660, 1997). In a separate study, the same gene cluster was identified and the lbgB (losB) gene was found to be required for transfer of the second sugar, D-glycero-D-manno-heptose (DD-Hep), of the major branch structure (Gibson et al., J. Bacteriol. 179:5062-5071, 1997). In this study, we identified the function of the neighboring upstream gene, lbgA, and found that it is necessary for addition of the third sugar in the dominant oligosaccharide branch, a galactose-linked beta1-->4, to the DD-Hep. LOS from an lbgA mutant and an lbgAB double mutant were isolated and were characterized by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, carbohydrate analysis, mass spectrometry, and nuclear magnetic resonance spectroscopy. The results showed that the mutant strains synthesize truncated LOS glycoforms that terminate after addition of the first glucose (lbgAB) or the disaccharide DD-Hepalpha1-->6Glcbeta1 (lbgA) that is attached to the heptose core. Both mutants show a significant reduction in the ability to adhere to human keratinocytes. Although minor differences were observed after two-dimensional gel electrophoresis of total proteins from the wild-type and mutant strains, the expression levels of the vast majority of proteins were unchanged, suggesting that the differences in adherence and invasion are due to differences in LOS. These studies add to the mounting evidence for a role of full-length LOS structures in the pathophysiology of H. ducreyi infection.
所有检测的杜克雷嗜血杆菌菌株都含有一种脂寡糖(LOS),它由一个单一但可变的分支寡糖组成,该分支寡糖从保守的3 - 磷酸化 - 3 - 脱氧 - D - 甘露 - 辛酮糖酸 - 脂质A核心的第一个庚糖(Hep - I)发出。在之前的一份报告中,描述了鉴定参与LOS生物合成的串联基因lbgA和lbgB(Stevens等人,《感染与免疫》65:651 - 660,1997年)。在另一项研究中,鉴定出了相同的基因簇,并且发现lbgB(losB)基因是主要分支结构的第二种糖,D - 甘油 - D - 甘露 - 庚糖(DD - Hep)转移所必需的(Gibson等人,《细菌学杂志》179:5062 - 5071,1997年)。在本研究中,我们鉴定了相邻上游基因lbgA的功能,发现它对于在优势寡糖分支中添加第三个糖,即与DD - Hep相连的半乳糖连接的β1→4是必需的。分离了来自lbgA突变体和lbgAB双突变体的LOS,并通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳、碳水化合物分析、质谱和核磁共振光谱对其进行了表征。结果表明,突变菌株合成了截短的LOS糖型,它们在添加第一个葡萄糖(lbgAB)或连接到庚糖核心的二糖DD - Hepα1→6Glcβ1(lbgA)后终止。两种突变体在黏附人角质形成细胞的能力上都有显著降低。尽管在对野生型和突变菌株的总蛋白进行二维凝胶电泳后观察到了微小差异,但绝大多数蛋白质的表达水平没有变化,这表明黏附与侵袭的差异是由于LOS的差异所致。这些研究进一步证明了全长LOS结构在杜克雷嗜血杆菌感染病理生理学中的作用。
