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[溶组织内阿米巴的微培养]

[Microcultures of Entamoeba].

作者信息

López-Griego L, Arroyo-Begovich A

机构信息

Departamento de Microbiología, Universidad Nacional Autónoma de México, D.F.

出版信息

Arch Invest Med (Mex). 1990;21 Suppl 1:119-22.

PMID:2136475
Abstract

The purpose of this study was the development of a microculture system for Entamoeba using ultrathin culture chambers, characterized by constant culture conditions, where the growing amebas can constantly be observed under the microscope, and which allows rapid variations in the characteristics of the culture medium, so as to determine the optimal conditions for growth and encystment of the ameba. After a lag phase the number of amebas increased following exponential kinetics. The E. invadens distribution in the culture chamber continued up to a total surface of (444 mm2) with in 7 days. On the whole E. invadens showed a tendency of not forming aggregates and growing until a confluent monolayer was reached. On the other hand, E. histolytica grew faster, covering the internal surface of the chamber in 5 days, and its growth went beyond a monolayer, since it covered all the internal walls, forming multiple aggregates. Encystment was induced in E. invadens by changing the feeding medium in the chamber for encystment medium. The encystment we observed was lower than that previously reported.

摘要

本研究的目的是开发一种用于溶组织内阿米巴的微培养系统,该系统采用超薄培养室,其特点是培养条件恒定,在显微镜下可不断观察生长中的阿米巴,并且能快速改变培养基特性,从而确定阿米巴生长和包囊形成的最佳条件。经过一个滞后期后,阿米巴数量呈指数动力学增加。侵袭内阿米巴在培养室内的分布持续到7天内总面积达到444平方毫米。总体而言,侵袭内阿米巴显示出不形成聚集体并生长直至达到汇合单层的趋势。另一方面,溶组织内阿米巴生长更快,在5天内覆盖培养室的内表面,并且其生长超出单层,因为它覆盖了所有内壁,形成多个聚集体。通过将培养室内的喂食培养基更换为包囊形成培养基来诱导侵袭内阿米巴形成包囊。我们观察到的包囊形成率低于先前报道的水平。

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