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通过琼脂糖-二乙氨基乙基离子交换色谱法纯化克氏锥虫循环后期锥鞭毛体,这是一种用于宿主-病原体相互作用研究的新方法。

Purification of Trypanosoma cruzi metacyclic trypomastigotes by ion exchange chromatography in sepharose-DEAE, a novel methodology for host-pathogen interaction studies.

作者信息

Cruz-Saavedra Lissa, Muñoz Marina, León Cielo, Patarroyo Manuel Alfonso, Arevalo Gabriela, Pavia Paula, Vallejo Gustavo, Carranza Julio César, Ramírez Juan David

机构信息

Universidad del Rosario, Facultad de Ciencias Naturales y Matemáticas, Programa de Biología, Grupo de Investigaciones Microbiológicas-UR (GIMUR), Bogotá, Colombia.

Molecular Biology and Immunology Department, Fundación Instituto de Inmunología de Colombia (FIDIC), Bogotá, Colombia; Universidad del Rosadio, School of Medicine and Health Sciences, Bogotá, Colombia.

出版信息

J Microbiol Methods. 2017 Nov;142:27-32. doi: 10.1016/j.mimet.2017.08.021. Epub 2017 Sep 1.

Abstract

Metacyclic trypomastigotes are essential for the understanding of the biology of Trypanosoma cruzi, the agent of Chagas disease. However, obtaining these biological stages in axenic medium is difficult. Techniques based on charge and density of the parasite during different stages have been implemented, without showing a high efficiency in the purification of metacyclic trypomastigotes. So far, there is no protocol implemented where sepharose-DEAE is used as a resin. Therefore, herein we tested its ability to purify metacyclic trypomastigotes in Liver Infusion Triptose (LIT) medium cultures. A simple, easy-to-execute and effective protocol based on ion exchange chromatography on Sepharose-DEAE resin for the purification of T. cruzi trypomastigotes is described. T. cruzi strains from the Discrete Typing Units (DTUs) I and II were used. The strains were harvested in LIT medium at a concentration of 1×10epimastigotes/mL. We calculated the time of trypomastigotes increment (TTI). Based on the data obtained, Ion exchange chromatography was performed with DEAE-sepharose resin. To verify the purity and viability of the trypomastigotes, a culture was carried out in LIT medium with subsequent verification with giemsa staining. To evaluate if the technique affected the infectivity of trypomastigotes, in vitro assays were performed in Vero cells and in vivo in ICR-CD1 mice. The technique allowed the purification of metacyclic trypomastigotes of other stages of T. cruzi in a percentage of 100%, a greater recovery was observed in cultures of 12days. There were differences regarding the recovery of metacyclic trypomastigotes for both DTUs, being DTU TcI the one that recovered a greater amount of these forms. The technique did not affect parasite infectivity in vitro or/and in vivo.

摘要

后循环型锥鞭毛体对于理解恰加斯病病原体克氏锥虫的生物学特性至关重要。然而,在无细胞培养基中获得这些生物学阶段很困难。基于寄生虫在不同阶段的电荷和密度的技术已经实施,但在纯化后循环型锥鞭毛体方面效率不高。到目前为止,还没有实施使用琼脂糖-二乙氨基乙基(sepharose-DEAE)作为树脂的方案。因此,在此我们测试了其在肝浸液胰蛋白胨(LIT)培养基培养物中纯化后循环型锥鞭毛体的能力。描述了一种基于琼脂糖-二乙氨基乙基树脂离子交换色谱法的简单、易于执行且有效的纯化克氏锥虫锥鞭毛体的方案。使用了来自离散分型单元(DTUs)I和II的克氏锥虫菌株。将菌株在LIT培养基中以1×10副鞭毛体/毫升的浓度收获。我们计算了锥鞭毛体增加时间(TTI)。根据获得的数据,用二乙氨基乙基琼脂糖树脂进行离子交换色谱。为了验证锥鞭毛体的纯度和活力,在LIT培养基中进行培养,随后用吉姆萨染色进行验证。为了评估该技术是否影响锥鞭毛体的感染性,在Vero细胞中进行了体外试验,并在ICR-CD1小鼠中进行了体内试验。该技术能够100%纯化克氏锥虫其他阶段的后循环型锥鞭毛体,在12天的培养物中观察到了更高的回收率。两个DTUs在后循环型锥鞭毛体的回收率方面存在差异,DTU TcI回收的这些形态的数量更多。该技术在体外或/和体内均不影响寄生虫的感染性。

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