人白蛋白溶液中内毒素和非内毒素热原的体外全血培养鉴别。

E J Pool, G Johaar, S James, I Petersen, P Bouic
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引用次数: 20

摘要

纯化的大肠杆菌内毒素、革兰氏阴性菌和革兰氏阳性菌通过全血培养诱导IL-6分泌。多粘菌素B浓度大于2 U/ml时,可完全抑制10 EU/ml内毒素引起的IL-6分泌。无内毒素时,多粘菌素B对白细胞分泌IL-6无影响。当多粘菌素B浓度小于1 U/ml时,对内毒素诱导的IL-6分泌的抑制作用依赖于多粘菌素B的浓度。多粘菌素B对枯草芽孢杆菌引起的IL-6分泌无影响,8 U/ml的多粘菌素B对大肠杆菌诱导的IL-6仅部分失活。我们还研究了兔热原测定法检测的两批人血清白蛋白(HSA)的热原性。4 U/ml的多粘菌素B对这些热原性HSA批次引起的IL-6分泌的抑制作用小于40%。加有纯化内毒素的HSA样品的内毒素活性均受到多粘菌素B的抑制,表明HSA不能保护内毒素免受多粘菌素B抑制。这些结果表明,这些HSA批次的热原性是由多粘菌素B抑制和非抑制部分引起的。本研究表明,除内毒素外的热原物质也可能污染成批的药品,使用鲎试剂(LAL)测定法获得的结果并不一定表明药品的热原状态。WBC热原测定法比LAL测定法具有更宽的灵敏度范围,是药品热原状态的更好指标。
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Differentiation between endotoxin and non-endotoxin pyrogens in human albumin solutions using an ex vivo whole blood culture assay.

Purified E.coli endotoxin, Gram negative bacteria and Gram positive bacteria induce IL-6 secretion by whole blood cultures (WBC's). Polymyxin B at concentrations greater than 2 U/ml completely inhibits IL-6 secretion caused by 10 EU/ml of endotoxin. Polymyxin B has no effect on IL-6 secretion by WBC's in the absence of endotoxin. The inhibition of endotoxin induced IL-6 secretion is Polymyxin B concentration dependent at concentrations less than 1 U/ml. IL-6 induction caused by E.coli is only partially inactivated by 8 U/ml Polymyxin B. Polymyxin B has no effect on IL-6 secretion caused by B.subtilis. Two pyrogenic batches of human serum albumin (HSA), as tested by the rabbit assay for pyrogens, were also investigated. Polymyxin B at 4 U/ml inhibits less than 40 % of IL-6 secretion caused by these pyrogenic HSA batches. All the endotoxin activity in HSA samples spiked with purified endotoxin is inhibited by Polymyxin B indicating that HSA does not protect endotoxin against Polymyxin B inhibition. These results indicate that the pyrogenicity of these HSA batches are caused by Polymyxin B inhibitable and non-inhibitable fractions. This study shows that pyrogenic substances other than endotoxin can contaminate batches of pharmaceutical products and that results obtained using the Limulus Amoebocyte Lysate (LAL) assay does not necessarily indicate the pyrogenic status of pharmaceutical products. The WBC assay for pyrogens, having a broader sensitivity range than the LAL assay, is a better indicator of the pyrogenic status of pharmaceutical products.

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