首页> 美国卫生研究院文献>The Journal of Biological Chemistry >Characterization of a Novel d-Glycero-d-talo-oct-2-ulosonic acid-substituted Lipid A Moiety in the Lipopolysaccharide Produced by the Acetic Acid Bacterium Acetobacter pasteurianus NBRC 3283
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Characterization of a Novel d-Glycero-d-talo-oct-2-ulosonic acid-substituted Lipid A Moiety in the Lipopolysaccharide Produced by the Acetic Acid Bacterium Acetobacter pasteurianus NBRC 3283

机译:醋酸菌醋杆菌NBRC 3283产生的脂多糖中新型d-甘油-d-talo-oct-2-ulosonic酸取代的脂质A部分的表征

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摘要

Acetobacter pasteurianus is an aerobic Gram-negative rod that is used in the fermentation process used to produce the traditional Japanese black rice vinegar kurozu. Previously, we found that a hydrophobic fraction derived from kurozu stimulates Toll-like receptors to produce cytokines. LPSs, particularly LPS from A. pasteurianus, are strong candidates for the immunostimulatory component of kurozu. The LPS of A. pasteurianus remains stable in acidic conditions during the 2 years of the abovementioned fermentation process. Thus, we hypothesized that its stability results from its structure. In this study, we isolated the LPS produced by A. pasteurianus NBRC 3283 bacterial cells and characterized the structure of its lipid A component. The lipid A moiety was obtained by standard weak acid hydrolysis of the LPS. However, the hydrolysis was incomplete because a certain proportion of the LPS contained acid-stable d-glycero-d-talo-oct-2-ulosonic acid (Ko) residues instead of the acid-labile 3-deoxy-d-manno-oct-2-ulosonic acid residues that are normally found in typical LPS. Even so, we obtained a Ko-substituted lipid A with a novel sugar backbone, α-Man(1–4)[α-Ko(2–6)]β-GlcN3N(1–6)α-GlcN(1–1)α-GlcA. Its reducing end GlcN(1-1)GlcA bond was also found to be quite acid-stable. Six fatty acids were attached to the backbone. Both the whole LPS and the lipid A moiety induced TNF-α production in murine cells via Toll-like receptor 4, although their activity was weaker than those of Escherichia coli LPS and lipid A. These results suggest that the structurally atypical A. pasteurianus lipid A found in this study remains stable and, hence, retains its immunostimulatory activity during acetic acid fermentation.
机译:巴氏醋杆菌是一种需氧革兰氏阴性棒,用于发酵过程中,该发酵过程用于生产传统的日本黑米醋黑醋。以前,我们发现衍生自kurozu的疏水部分会刺激Toll样受体产生细胞因子。 LPS,特别是来自巴斯德曲霉的LPS,是黑醋栗免疫刺激成分的强候选者。在上述发酵过程的两年中,巴氏曲霉的LPS在酸性条件下保持稳定。因此,我们假设其稳定性源于其结构。在这项研究中,我们分离了由巴斯德曲霉NBRC 3283细菌细胞产生的LPS,并表征了其脂质A组分的结构。通过LPS的标准弱酸水解获得脂质A部分。但是,水解是不完全的,因为一定比例的LPS含有酸稳定的d-甘油-d-talo-oct-2-ulosonic酸(Ko)残基,而不是酸不稳定的3-deoxy-d-manno-oct通常在典型的LPS中发现的-2-磺酸残基。即便如此,我们还是获得了带有新型糖主链α-Man(1-4)[α-Ko(2-6)]β-GlcN3N(1-6)α-GlcN(1-1的Ko取代脂质A。 )α-GlcA。还发现其还原端GlcN(1-1)GlcA键是相当酸稳定的。六个脂肪酸附着在主链上。整个LPS和脂质A部分都通过Toll样受体4诱导鼠细胞中TNF-α的产生,尽管它们的活性比大肠杆菌LPS和脂质A弱。这些结果表明,结构上非典型的巴斯德曲霉脂质在这项研究中发现的保持稳定,因此,在乙酸发酵过程中保持其免疫刺激活性。

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