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Quantitative assessment of the proliferation of the protozoan parasite Perkinsus marinus using a bioluminescence assay for ATP content

机译:使用生物发光法测定ATP含量定量评估原生动物寄生虫Perkinsus marinus的增殖

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摘要

class="kwd-title">Keywords: Antibiotics, Herbicides, Perkinsus, Plastid, Protozoan class="head no_bottom_margin" id="idm139737656644416title">AbstractPerkinsus marinus is a protozoan parasite that causes “Dermo” disease in the eastern oyster Crasssostrea virginica in coastal areas of the USA. Until now, intervention strategies against the parasite have found limited success, and Dermo still remains one of the main hurdles for the restoration of oyster populations. We adapted a commercial adenosine tri-phosphate (ATP) content-based assay to assess the in vitro proliferation of P. marinus in a 96-well plate format, and validated the method by measuring the effects of potential anti-proliferative compounds. The sensitivity (1.5–3.1 × 104 cells/well), linearity (R2 = 0.983), and signal stability (60 min) support the reliability of the assay for assessing cell proliferation. Validation of the assay by culturing P. marinus in the presence of increasing concentrations of triclosan showed a dose–response profile. The IC50 value obtained was higher than that reported earlier, possibly due to the use of different viability assay methods and a different P. marinus strain. The antibiotics G418 and tetracycline and the herbicide fluridone were active against P. marinus proliferation; the IC50 of chloramphenicol, ciprofloxacin, and atrazine was relatively high suggesting either off-target effects or inability to reach the targets. The validation of the ATP-based assay, together with significant advantages of the Perkinsus culture methodology (homogeneity, reproducibility, and high cell densities), underscores the value of this assay for developing high-throughput screens for the identification of novel leader compounds against Perkinsus species, and most importantly, for the closely-related apicomplexan parasites.
机译:<!-fig ft0-> <!-fig @ position =“ anchor” mode =文章f4-> <!-fig mode =“ anchred” f5-> <!-fig / graphic | fig / alternatives / graphic mode =“ anchored” m1-> class =“ kwd-title”>关键字:抗生素,除草剂,Perkinsus,Plastid,原生动物 class =“ head no_bottom_margin” id =“ idm139737656644416416title “>摘要海鲈是一种原生动物寄生虫,在美国沿海地区的东部牡蛎Crasssostrea virginica引起“ Dermo”病。迄今为止,针对寄生虫的干预策略仅取得了有限的成功,Dermo仍然是恢复牡蛎种群的主要障碍之一。我们采用了一种基于三磷酸腺苷(ATP)含量的商业化检测方法,以96孔板的形式评估了海藻的体外增殖,并通过测量潜在的抗增殖化合物的效果验证了该方法。灵敏度(1.5–3.1×10 4 细胞/孔),线性度(R 2 = 0.983)和信号稳定性(60分钟)支持测定的可靠性评估细胞增殖。通过在浓度增加的三氯生存在下培养海藻假单胞菌来验证该测定方法的剂量反应曲线。获得的IC50值高于早先报告的IC50值,这可能是由于使用了不同的活力测定方法和不同的体育假单胞菌菌株。抗生素G418和四环素以及除草剂氟啶酮对海藻的增殖具有活性。氯霉素,环丙沙星和阿特拉津的IC50值相对较高,表明脱靶效应或无法达到靶点。基于ATP的测定方法的验证以及珀金斯氏菌培养方法的显着优势(均质性,可重复性和高细胞密度),突显了该测定法对于开发高通量筛选以鉴定针对珀金氏菌的新型前导化合物的价值物种,最重要的是与紧密相关的apicomplexan寄生虫有关。

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