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Characterization of the native form of anthrax lethal factor for use in the toxin neutralization assay

机译:炭疽致死因子的天然形式的表征用于毒素中和测定

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The cell-based anthrax toxin neutralization assay (TNA) is used to determine functional antibody titers of sera from animals and humans immunized with anthrax vaccines. The anthrax lethal toxin is a critical reagent of the TNA composed of protective antigen (PA) and lethal factor (LF), which are neutralization targets of serum antibodies. Cytotoxic potency of recombinant LF (rLF) lots can vary substantially, causing a challenge in producing a renewable supply of this reagent for validated TNAs. To address this issue, we characterized a more potent rLF variant (rLF-A) with the exact native LF amino acid sequence that lacks the additional N-terminal histidine and methionine residues present on the commonly used form of rLF (rLF-HMA) as a consequence of the expression vector. rLF-A can be used at 4 to 6 ng/ml (in contrast to 40 ng/ml rLF-HMA) with 50 ng/ml recombinant PA (rPA) to achieve 95 to 99% cytotoxicity. In the presence of 50 ng/ml rPA, both rLF-A and rLF-HMA allowed for similar potencies (50% effective dilution) among immune sera in the TNA. rPA, but not rLF, was the dominant factor in determining potency of serum samples containing anti-PA antibodies only or an excess of anti-PA relative to anti-rLF antibodies. Such anti-PA content is reflected in immune sera derived from most anthrax vaccines in development. These results support that 7- to 10-fold less rLF-A can be used in place of rLF-HMA without changing TNA serum dilution curve parameters, thus extending the use of a single rLF lot and a consistent, renewable supply.
机译:基于细胞的炭疽毒素中和测定(TNA)用于确定用炭疽疫苗免疫的动物和人类血清的功能抗体滴度。炭疽致死毒素是由保护性抗原(PA)和致死因子(LF)组成的TNA的关键试剂,它们是血清抗体的中和靶标。重组LF(RLF)批次的细胞毒性效力可能会有很大差异,从而在产生该试剂的可再生供应中构成了挑战,以用于验证的TNA。为了解决这个问题,我们用精确的天然LF氨基酸序列表征了更有效的RLF变体(RLF-A),该序列缺乏在常用的RLF(RLF-HMA)上存在的其他N末端组氨酸和蛋氨酸残基,作为RLF(RLF-HMA)表达载体的结果。 RLF-A可在4至6 ng/mL(与40 ng/ml RLF-HMA相比)中使用50 ng/ml重组PA(RPA),以达到95%至99%的细胞毒性。在有50 ng/mL RPA的情况下,RLF-A和RLF-HMA都允许在TNA中的免疫血清中具有相似的效力(有效稀释50%)。 RPA(而不是RLF)是仅相对于抗RLF抗体的抗Pa抗体或过量抗PA的血清样品的效力。这种抗PA含量反映在发育中大多数炭疽疫苗的免疫血清中。这些结果支持,可以使用RLF-HMA的RLF-A少7-10倍,而无需更改TNA血清稀释曲线参数,从而扩展了单个RLF批次的使用和一致的可再生供应。

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