Literature DB >> 17510256

Use of a colorimetric assay to measure differences in cytotoxicity of Mycobacterium tuberculosis strains.

Jorge Castro-Garza1, Hugo B Barrios-García2,1, Delia Elva Cruz-Vega1, Salvador Said-Fernández1, Pilar Carranza-Rosales1, Carmen A Molina-Torres3, Lucio Vera-Cabrera3.   

Abstract

Several techniques have been used to quantify the cytotoxicity produced by Mycobacterium tuberculosis bacilli on cell monolayers; however, they are semi-quantitative or time consuming. Herein, a method based on crystal violet (CV) uptake by THP-1 cell monolayers is described. This colorimetric method quantifies the cytotoxic effect as a function of the number of remaining cells after the infection with M. tuberculosis. Since this micro-organism is not stained by the dye, it does not produce a background that affects absorbance readings. As determined by CV assay (CVA), M. tuberculosis strain H37Rv destroyed 10.5 % of THP-1 cell monolayers at 24 h and 50.52 % at 72 h, while M. tuberculosis strains lacking the complete phospholipase C locus produced a reduced cytotoxic effect. The damage estimated by microscopy corresponded to the effect quantified by CVA. The results show that the use of CVA is a rapid, sensitive and reliable quantitative assay to measure the cytotoxicity of different M. tuberculosis strains.

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Year:  2007        PMID: 17510256     DOI: 10.1099/jmm.0.46915-0

Source DB:  PubMed          Journal:  J Med Microbiol        ISSN: 0022-2615            Impact factor:   2.472


  7 in total

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7.  Modeling tuberculosis pathogenesis through ex vivo lung tissue infection.

Authors:  Pilar Carranza-Rosales; Irma Edith Carranza-Torres; Nancy Elena Guzmán-Delgado; Gerardo Lozano-Garza; Licet Villarreal-Treviño; Carmen Molina-Torres; Javier Vargas Villarreal; Lucio Vera-Cabrera; Jorge Castro-Garza
Journal:  Tuberculosis (Edinb)       Date:  2017-09-12       Impact factor: 3.131

  7 in total

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