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首页> 美国卫生研究院文献>Springer Open Choice >High-sensitivity MALDI-TOF MS quantification of anthrax lethal toxin for diagnostics and evaluation of medical countermeasures
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High-sensitivity MALDI-TOF MS quantification of anthrax lethal toxin for diagnostics and evaluation of medical countermeasures

机译:炭疽致死毒素的高灵敏度MALDI-TOF MS定量用于诊断和评估医学对策

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Inhalation anthrax has a rapid progression and high fatality rate. Pathology and death from inhalation of Bacillus anthracis spores are attributed to the actions of secreted protein toxins. Protective antigen (PA) binds and imports the catalytic component lethal factor (LF), a zinc endoprotease, and edema factor (EF), an adenylyl cyclase, into susceptible cells. PA-LF is termed lethal toxin (LTx) and PA-EF, edema toxin. As the universal transporter for both toxins, PA is an important target for vaccination and immunotherapeutic intervention. However, its quantification has been limited to methods of relatively low analytic sensitivity. Quantification of LTx may be more clinically relevant than LF or PA alone because LTx is the toxic form that acts on cells. A method was developed for LTx-specific quantification in plasma using anti-PA IgG magnetic immunoprecipitation of PA and quantification of LF activity that co-purified with PA. The method was fast (<4 h total time to detection), sensitive at 0.033 ng/mL LTx in plasma for the fast analysis (0.0075 ng/mL LTx in plasma for an 18 h reaction), precise (6.3–9.9 % coefficient of variation), and accurate (0.1–12.7 %error; n ≥ 25). Diagnostic sensitivity was 100 % (n = 27 animal/clinical cases). Diagnostic specificity was 100 % (n = 141). LTx was detected post-antibiotic treatment in 6/6 treated rhesus macaques and 3/3 clinical cases of inhalation anthrax and as long as 8 days post-treatment. Over the course of infection in two rhesus macaques, LTx was first detected at 0.101 and 0.237 ng/mL at 36 h post-exposure and increased to 1147 and 12,107 ng/mL in late-stage anthrax. This demonstrated the importance of LTx as a diagnostic and therapeutic target. This method provides a sensitive, accurate tool for anthrax toxin detection and evaluation of PA-directed therapeutics.>Graphical AbstractMethod schematic for analysis of anthrax lethal toxin activity by ID-MALDI-TOF MS
机译:吸入性炭疽病发展迅速,死亡率高。吸入炭疽芽孢杆菌的病理学和死亡归因于分泌的蛋白质毒素的作用。保护性抗原(PA)结合并导入催化成分致死因子(LF)(锌内切蛋白酶)和水肿因子(EF)(腺苷酸环化酶)并将其导入易感细胞。 PA-LF被称为致命毒素(LTx)和PA-EF水肿毒素。作为两种毒素的通用转运蛋白,PA是疫苗接种和免疫治疗干预的重要目标。但是,其量化仅限于分析灵敏度相对较低的方法。 LTx的量化可能比单独使用LF或PA更具临床相关性,因为LTx是作用于细胞的有毒形式。开发了一种使用抗PA IgG磁性免疫沉淀PA和定量与PA共纯化的LF活性进行血浆LTx特异性定量的方法。该方法快速(总检测时间<4小时),对血浆中的0.033 ng / mL LTx敏感,可进行快速分析(对于18小时的反应,在血浆中为0.0075 ng / mL LTx),精确(6.3-9.9%的系数差异),并且准确(误差为0.1-12.7%;n≥≥25)。诊断敏感性为100%(n = 27例动物/临床病例)。诊断特异性为100%(n = 141)。在接受抗生素治疗的6/6恒河猴和3/3吸入性炭疽的临床病例中,以及治疗后长达8天,均检测到LTx。在两只猕猴的感染过程中,暴露后36小时首次检测到LTx的浓度为0.101和0.237 ng / mL,后期炭疽中的LTx浓度增至1147和12,107 ng / mL。这证明了LTx作为诊断和治疗靶标的重要性。此方法为炭疽毒素检测和PA定向治疗提供了灵敏,准确的工具。<!-fig ft0-> <!-fig @ position =“ anchor” mode = f4-> <!- -fig mode =“ anchored” f5-> >图形摘要<!-fig / graphic | fig / alternatives / graphic mode =“ anchored” m1-> <!-标题a7->方法示意图ID-MALDI-TOF MS分析炭疽致死毒素活性

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