传统百日咳疫苗中的脂多糖

P. Ibsen , S. Møller , I. Heron
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引用次数: 12

摘要

对丹麦产的4株百日咳疫苗(3803、3825、3843和3860)和纯化菌株3803的细胞超声脂多糖(LPS,内毒素)进行银染色分析,结果表明:纯化菌株3803的细胞超声脂多糖(LPS,内毒素)谱图完全一致。LPS谱显示一个显性的褐色LPS II带和一个次要的、快速迁移的黑色LPS I带。然而,在制备纯化LPS时,LPS I与LPS II的比例与细胞超声略有不同。利用标记LPS,估计LPS I和LPS II的分子量分别为5.4和6.0 kD。对7批全细胞百日咳疫苗进行鲎试剂检测,发现LPS含量为0.9 ~ 2.8 μg /ml。不同菌株在相似稀释度下LPS含量无显著差异。此外,研究了游离和细胞结合LPS在四种百日咳疫苗中的分布。大部分LPS以游离LPS的形式存在。在几个月内,LPS和百日咳毒素(Pt)在新鲜杀死百日咳制剂中的释放过程被跟踪。在最初的几周内,35-50%的LPS被释放,5-6个月后,60-80%的LPS被释放。相比之下,在实验期间,只有不到10%的生物活性百日咳毒素被释放。讨论了在不降低保护价值的情况下,通过减少游离LPS的量来生产更安全的全细胞百日咳疫苗的可能性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Lipopolysaccharides in a traditional pertussis vaccine

Analysis of the lipopolysaccharide (LPS, endotoxin) in cell sonicates of four Danish vaccine strains of Bordetella pertussis (3803, 3825, 3843 and 3860) and of purified strain 3803 LPS in sodium dodecyl sulphate-polyacrylamide gel electrophoresis by silver staining, showed identical profiles. The LPS profile revealed a dominant, brownish LPS II band and a minor, faster-migrating, black-stained LPS I band. However, the ratio of LPS I to LPS II in the preparation of purified LPS differed slightly from the cell sonicates. Using marker LPS, the molecular weights of LPS I and LPS II were estimated at 5·4 and 6·0 kD, respectively. Seven different lots of whole cell pertussis vaccine were assayed for LPS in the Limulus Amoebocyte Lysate test and were found to contain 0·9 – 2·8 μg LPS/ml. No significant difference in the content of LPS in similar dilutions of the individual strains was observed. In addition, the distribution of free and cell-bound LPS in four pertussis vaccines was investigated. Most of the LPS was found to exist as free LPS. During several months, the course of both LPS and pertussis toxin (Pt) release in freshly killed B. pertussis preparations was followed. In the first few weeks, 35–50% of the LPS was released and after 5–6 months of storage 60–80% had been released. In contrast, less than 10% of the biologically active pertussis toxin was released during the experimental period. The possibility of producing a safer whole cell pertussis vaccine by reducing the amount of free LPS without reducing the protective value correspondingly is discussed.

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