Screening the Global Health Priority Box against Plasmodium berghei liver stage parasites using an inexpensive luciferase detection protocol.

IF 2.4 3区 医学 Q3 INFECTIOUS DISEASES
Gia-Bao Nguyen, Caitlin A Cooper, Olivia McWhorter, Ritu Sharma, Anne Elliot, Anthony Ruberto, Rafael Freitas, Ashutosh K Pathak, Dennis E Kyle, Steven P Maher
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引用次数: 0

Abstract

Background: Malaria, a disease caused by parasites of the genus Plasmodium, continues to impact many regions globally. The rise in resistance to artemisinin-based anti-malarial drugs highlights the need for new treatments. Ideally, new anti-malarials will kill the asymptomatic liver stages as well as the symptomatic blood stages. While blood stage screening assays are routine and efficient, liver stage screening assays are more complex and costly. To decrease the cost of liver stage screening, a previously reported luciferase detection protocol requiring only common laboratory reagents was adapted for testing against luciferase-expressing Plasmodium berghei liver stage parasites.

Methods: After optimizing cell lysis conditions, the concentration of reagents, and the density of host hepatocytes (HepG2), the protocol was validated with 28 legacy anti-malarials to show this simple protocol produces a stable signal useful for obtaining quality small molecule potency data similar to that obtained from a high content imaging endpoint. The protocol was then used to screen the Global Health Priority Box (GHPB) and confirm the potency of hits in dose-response assays. Selectivity was determined using a galactose-based, 72 h HepG2 assay to avoid missing mitochondrial-toxic compounds due to the Crabtree effect. Receiver-operator characteristic plots were used to retroactively characterize the screens' predictive value.

Results: Optimal luciferase signal was achieved using a lower HepG2 seed density (5 × 103 cells/well of a 384-well microtitre plate) compared to many previously reported luciferase-based screens. While producing lower signal compared to a commercial alternative, this luciferase detection method was found much more stable, with a > 3 h half-life, and robust enough for producing dose-response plots with as few as 500 sporozoites/well. A screen of the GHPB resulted in 9 hits with selective activity against P. berghei liver schizonts, including MMV674132 which exhibited 30.2 nM potency. Retrospective analyses show excellent predictive value for both anti-malarial activity and cytotoxicity.

Conclusions: This method is suitable for high-throughput screening at a cost nearly 20-fold less than using commercial luciferase detection kits, thereby enabling larger liver stage anti-malarial screens and hit optimization make-test cycles. Further optimization of the hits detected using this protocol is ongoing.

利用廉价的荧光素酶检测方案筛查全球健康优先箱中的贝氏疟原虫肝阶段寄生虫。
背景:疟疾是一种由疟原虫属寄生虫引起的疾病,继续影响着全球许多地区。青蒿素类抗疟药物抗药性的增加凸显了对新疗法的需求。理想的情况是,新的抗疟疾药物既能杀死无症状的肝期疟原虫,也能杀死有症状的血期疟原虫。血液阶段的筛查测定是常规且高效的,而肝脏阶段的筛查测定则更为复杂和昂贵。为了降低肝阶段筛查的成本,我们对之前报道的只需普通实验室试剂的荧光素酶检测方案进行了改良,用于检测表达荧光素酶的伯格氏疟原虫肝阶段寄生虫:在对细胞裂解条件、试剂浓度和宿主肝细胞(HepG2)密度进行优化后,用 28 种传统的抗疟疾药物对该方案进行了验证,结果表明这种简单的方案能产生稳定的信号,有助于获得高质量的小分子药效数据,类似于从高含量成像终点获得的数据。随后,该方案被用于筛选全球健康优先药盒(GHPB),并在剂量反应试验中确认命中药物的效力。使用基于半乳糖的 72 h HepG2 试验确定选择性,以避免因克拉布特里效应而遗漏线粒体毒性化合物。使用接收器-运算器特征图来追溯筛选的预测价值:与之前报道的许多基于荧光素酶的筛选方法相比,使用较低的 HepG2 种子密度(384 孔微滴定板 5 × 103 个细胞/孔)就能获得最佳荧光素酶信号。这种荧光素酶检测方法虽然产生的信号比商业替代方法低,但却更加稳定,半衰期大于 3 小时,而且足够强大,可以在每孔只有 500 个孢子的情况下绘制剂量反应图。GHPB 筛选出了 9 种对伯格希氏虫肝裂殖体具有选择性活性的药物,其中 MMV674132 具有 30.2 nM 的效力。回顾性分析表明,该方法对抗疟活性和细胞毒性都有很好的预测价值:这种方法适用于高通量筛选,其成本比使用商业荧光素酶检测试剂盒低近 20 倍,因此可以进行更大规模的肝脏期抗疟筛选和新药优化制造-测试循环。目前正在对使用该方案检测到的新药进行进一步优化。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Malaria Journal
Malaria Journal 医学-寄生虫学
CiteScore
5.10
自引率
23.30%
发文量
334
审稿时长
2-4 weeks
期刊介绍: Malaria Journal is aimed at the scientific community interested in malaria in its broadest sense. It is the only journal that publishes exclusively articles on malaria and, as such, it aims to bring together knowledge from the different specialities involved in this very broad discipline, from the bench to the bedside and to the field.
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