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一种使用转染红色荧光蛋白的亚马逊利什曼原虫进行的体外药物筛选替代试验。

An alternative in vitro drug screening test using Leishmania amazonensis transfected with red fluorescent protein.

机构信息

Centro de Pesquisas René Rachou, Fundação Oswaldo Cruz/FIOCRUZ, Belo Horizonte, MG, Brazil.

出版信息

Diagn Microbiol Infect Dis. 2013 Mar;75(3):282-91. doi: 10.1016/j.diagmicrobio.2012.11.018. Epub 2013 Jan 10.

Abstract

Fluorescent and colorimetric reporter genes are valuable tools for drug screening models, since microscopy is labor intensive and subject to observer variation. In this work, we propose a fluorimetric method for drug screening using red fluorescent parasites. Fluorescent Leishmania amazonensis were developed after transfection with integration plasmids containing either red (RFP) or green fluorescent protein (GFP) genes. After transfection, wild-type (LaWT) and transfected (LaGFP and LaRFP) parasites were subjected to flow cytometry, macrophage infection, and tests of susceptibility to current antileishmanial agents and propranolol derivatives previously shown to be active against Trypanosoma cruzi. Flow cytometry analysis discriminated LaWT from LaRFP and LaGFP parasites, without affecting cell size or granulosity. With microscopy, transfection with antibiotic resistant genes was not shown to affect macrophage infectivity and susceptibility to amphotericin B and propranolol derivatives. Retention of fluorescence remained in the intracellular amastigotes in both LaGFP and LaRFP transfectants. However, detection of intracellular RFP parasites was only achieved in the fluorimeter. Murine BALB/c macrophages were infected with LaRFP parasites, exposed to standard (meglumine antimoniate, amphotericin B, Miltefosine, and allopurinol) and tested molecules. Although it was possible to determine IC(50) values for 4 propranolol derivatives (1, 2b, 3, and 4b), all compounds were considered inactive. This study is the first to develop a fluorimetric drug screening test for L. amazonensis RFP. The fluorimetric test was comparable to microscopy with the advantage of being faster and not requiring manual counting.

摘要

荧光和比色报告基因是药物筛选模型的有价值工具,因为显微镜检查既费力又容易受到观察者的变化影响。在这项工作中,我们提出了一种使用红色荧光寄生虫进行药物筛选的荧光测定法。在转染包含红色(RFP)或绿色荧光蛋白(GFP)基因的整合质粒后,开发了荧光发光型利什曼原虫。转染后,野生型(LaWT)和转染的(LaGFP 和 LaRFP)寄生虫进行了流式细胞术分析、巨噬细胞感染以及对当前抗利什曼原虫药物和先前显示对克氏锥虫有效的普萘洛尔衍生物的敏感性测试。流式细胞术分析区分了 LaWT 与 LaRFP 和 LaGFP 寄生虫,而不影响细胞大小或颗粒度。通过显微镜观察,抗生素抗性基因的转染并未显示出对巨噬细胞感染性和两性霉素 B 及普萘洛尔衍生物敏感性的影响。在 LaGFP 和 LaRFP 转染子中,荧光在细胞内无鞭毛体中仍然保留。然而,仅在荧光计中检测到细胞内 RFP 寄生虫。用 LaRFP 寄生虫感染小鼠 BALB/c 巨噬细胞,暴露于标准药物(葡甲胺锑酸钠、两性霉素 B、米替福新和别嘌呤醇)和测试分子。虽然可以确定 4 种普萘洛尔衍生物(1、2b、3 和 4b)的 IC50 值,但所有化合物均被认为无效。这项研究是首次开发针对 L. amazonensis RFP 的荧光药物筛选测试。荧光测定法与显微镜检查相当,具有更快且不需要手动计数的优势。

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