A Three-Dimensional Lung Cell Model to Leptospira Virulence Investigations

被引:0
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作者
Camila L. Campos
Luciana R. Gomes
Ambart E. Covarrubias
Ellen E. Kato
Gisele G. Souza
Silvio A. Vasconcellos
Marcos B. Heinemann
Elizabeth A. L. Martins
Paulo L. Ho
Renata M. A. Da Costa
Josefa B. Da Silva
机构
[1] Instituto Butantan,Laboratório de Bacteriologia
[2] Instituto Butantan,Laboratório de Ciclo Celular
[3] Universidad San Sebastian,Center for Research on Toxins, Immune
[4] Instituto Butantan,Response and Cell Signaling (CeTICS)
[5] Universidade de São Paulo,Facultad de Ciencias de la Salud, Escuela de Tecnología Médica
[6] Instituto Butantan,Laboratorio de Fisiopatologia
[7] Instituto Butantan,Laboratório de Zoonoses Bacterianas, Faculdade de Medicina Veterinária e Zootecnia
[8] Global Antibiotics Research and Development Partnership (GARDP),Laboratório de Biológicos Recombinantes
来源
Current Microbiology | 2022年 / 79卷
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摘要
Leptospirosis is a worldwide zoonosis and a serious public health threat in tropical and subtropical areas. The etiologic agents of leptospirosis are pathogenic spirochetes from the genus Leptospira. In severe cases, patients develop a pulmonary hemorrhage that is associated with high fatality rates. Several animal models were established for leptospirosis studies, such as rodents, dogs, and monkeys. Although useful to study the relationship among Leptospira and its hosts, the animal models still exhibit economic and ethical limitation reasons and do not fully represent the human infection. As an attempt to bridge the gap between animal studies and clinical information from patients, we established a three-dimensional (3-D) human lung cell culture for Leptospira infection. We show that Leptospira is able to efficiently infect the cell lung spheroids and also to infiltrate in deeper areas of the cell aggregates. The ability to infect the 3-D lung cell aggregates was time-dependent. The 3-D spheroids infection occurred up to 120 h in studies with two serovars, Canicola and Copenhageni. We standardized the number of bacteria in the initial inoculum for infection of the spheroids and we also propose two alternative culture media conditions. This new approach was validated by assessing the expression of three genes of Leptospira related to virulence and motility. The transcripts of these genes increased in both culture conditions, however, in higher rates and earlier times in the 3-D culture. We also assessed the production of chemokines by the 3-D spheroids before and after Leptospira infection, confirming induction of two of them, mainly in the 3-D spheroids. Chemokine CCL2 was expressed only in the 3-D cell culture. Increasing of this chemokine was observed previously in infected animal models. This new approach provides an opportunity to study the interaction of Leptospira with the human lung epithelium in vitro.
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