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铜绿假单胞菌脂多糖化学成分的进一步研究。

Further studies of the chemical composition of the lipopolysaccharide of Pseudomonas aeruginosa.

作者信息

Chester I R, Gray G W, Wilkinson S G

出版信息

Biochem J. 1972 Jan;126(2):395-407. doi: 10.1042/bj1260395.

Abstract
  1. Qualitative and quantitative analytical results for the lipopolysaccharide from acetone-dried cells of Pseudomonas aeruginosa (N.C.T.C. 1999) are presented and possible contamination of the material with nucleic acid was further examined. 2. Additional sugars detected (only in large-scale hydrolysates) were mannose and arabinose; traces of spermidine and putrescine were also found. 3. The heptose component is l-glycero-d-mannoheptose. 4. The thiobarbituric acid-positive component is a 3-deoxy-2-octulonic acid, of which only 35-40% links lipid A to the polysaccharide. This linkage is not broken by hydrolysis with acetic acid up to 0.08m. 5. Liberation of lipid A required hydrolysis with 0.1m-hydrochloric acid, which substantially degraded the polysaccharide moiety. 6. Fractions obtained from the degraded polysaccharide by high-voltage electrophoresis were examined; in these, the alanine/galactosamine molar ratio is approx. 1. 7. Hydrazinolysis of whole lipopolysaccharide showed that at least 40% of the alanine is in amide linkage, possibly with galactosamine. 8. Lipid A, solubilized by alkaline methanolysis was fractionated; most of the phosphorus of the higher-molecular-weight fractions was released as P(i) by a phosphomonoesterase. 9. Hydrazinolysis of lipid A destroyed approx. 80% of the glucosamine, and glycosidically linked glucosamine oligosaccharides could not be isolated.
摘要
  1. 本文给出了铜绿假单胞菌(N.C.T.C. 1999)丙酮干燥细胞中脂多糖的定性和定量分析结果,并进一步检测了该物质可能被核酸污染的情况。2. 检测到的其他糖类(仅在大规模水解产物中)为甘露糖和阿拉伯糖;还发现了痕量的亚精胺和腐胺。3. 庚糖成分为L-甘油-D-甘露庚糖。4. 硫代巴比妥酸阳性成分是3-脱氧-2-辛酮酸,其中只有35 - 40%将类脂A与多糖相连。用浓度高达0.08m的乙酸水解不会破坏这种连接。5. 释放类脂A需要用0.1m盐酸水解,这会使多糖部分大量降解。6. 对通过高压电泳从降解的多糖中获得的组分进行了检测;其中丙氨酸/半乳糖胺的摩尔比约为1。7. 对整个脂多糖进行肼解表明,至少40%的丙氨酸处于酰胺键中,可能与半乳糖胺相连。8. 用碱性甲醇解溶解的类脂A进行了分级分离;较高分子量级分中的大部分磷通过磷酸单酯酶以无机磷酸(P(i))的形式释放出来。9. 对类脂A进行肼解破坏了约80%的葡糖胺,且无法分离出糖苷键连接的葡糖胺寡糖。

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