TY - JOUR
T1 - Standardization of a fluorescent-based quantitative adhesion assay to study attachment of Taenia solium oncosphere to epithelial cells in vitro
AU - Chile, Nancy
AU - Evangelista, Julio
AU - Gilman, Robert H.
AU - Arana, Yanina
AU - Palma, Sandra
AU - Sterling, Charles R.
AU - Garcia, Hector H.
AU - Gonzalez, Armando
AU - Verastegui, Manuela
N1 - Funding Information:
This work was supported by The Fogarty International Clinical Research Scholars and Fellows Program at Vanderbilt University ( R24 TW007988 ), Bill and Melinda Gates Foundation — Cysticercosis Elimination in Peru (grants 23981 and 33848 ), 5D43TW006581 National Institutes of Health “Infectious Diseases Training Program in Peru”, Training Grant ( FIC/NIH D43 TW001140 ) and the RG-ER anonymous fund for Tropical Research. We thank Dr. Karen Alroy for revising and editing the manuscript, Dr. Eric Deharo and Dr. Yanick Estevez for help with the use of the Chamaleon V Microplate Reader, and the technical assistance of J.B. Phu, D. and Sara.
PY - 2012/2/28
Y1 - 2012/2/28
N2 - To fully understand the preliminary stages of Taenia solium oncosphere attachment in the gut, adequate tools and assays are necessary to observe and quantify this event that leads to infection. A fluorescent-based quantitative adhesion assay, using biotinylated activated-oncospheres and monolayers of Chinese hamster ovary cells (CHO-K1) or human intestinal monolayer cells (INT-407, HCT-8 or HT-29), was developed to study initial events during the infection of target cells and to rapidly quantify the in vitro adhesion of T. solium oncospheres. Fluorescein streptavidin was used to identify biotinylated activated-oncospheres adhered to cells. This adherence was quantified using an automated fluorescence plate reader, and the results were expressed as fluorescence intensity values. A series of three assays were performed. The first was to identify the optimum number of biotinylated activated-oncospheres to be used in the adhesion assay. The goal of the second assay was to validate this novel method with the established oncosphere-binding system using the immunofluorescent-antibody assay (IFA) method to quantify oncosphere adhesion. A total of 10,000 biotinylated activated-oncospheres were utilized to assess the role of sera and laminin (LM) in oncosphere adherence to a CHO-K1 cell monolayer. The findings that sera and LM increase the adhesion of oncospheres to monolayer cells were similar to results that were previously obtained using the IFA method. The third assay compared the adherence of biotinylated activated-oncospheres to different types of human intestinal monolayer cells. In this case, the fluorescence intensity was greatest when using the INT-407 cell monolayer. We believe this new method of quantification offers the potential for rapid, large-scale screening to study and elucidate specific molecules and mechanisms involved in oncosphere-host cell attachment.
AB - To fully understand the preliminary stages of Taenia solium oncosphere attachment in the gut, adequate tools and assays are necessary to observe and quantify this event that leads to infection. A fluorescent-based quantitative adhesion assay, using biotinylated activated-oncospheres and monolayers of Chinese hamster ovary cells (CHO-K1) or human intestinal monolayer cells (INT-407, HCT-8 or HT-29), was developed to study initial events during the infection of target cells and to rapidly quantify the in vitro adhesion of T. solium oncospheres. Fluorescein streptavidin was used to identify biotinylated activated-oncospheres adhered to cells. This adherence was quantified using an automated fluorescence plate reader, and the results were expressed as fluorescence intensity values. A series of three assays were performed. The first was to identify the optimum number of biotinylated activated-oncospheres to be used in the adhesion assay. The goal of the second assay was to validate this novel method with the established oncosphere-binding system using the immunofluorescent-antibody assay (IFA) method to quantify oncosphere adhesion. A total of 10,000 biotinylated activated-oncospheres were utilized to assess the role of sera and laminin (LM) in oncosphere adherence to a CHO-K1 cell monolayer. The findings that sera and LM increase the adhesion of oncospheres to monolayer cells were similar to results that were previously obtained using the IFA method. The third assay compared the adherence of biotinylated activated-oncospheres to different types of human intestinal monolayer cells. In this case, the fluorescence intensity was greatest when using the INT-407 cell monolayer. We believe this new method of quantification offers the potential for rapid, large-scale screening to study and elucidate specific molecules and mechanisms involved in oncosphere-host cell attachment.
KW - Biotinylation
KW - Epithelial cells
KW - Quantitative adhesion assay
KW - Taenia solium oncosphere
UR - http://www.scopus.com/inward/record.url?scp=84856527545&partnerID=8YFLogxK
U2 - 10.1016/j.jim.2011.12.001
DO - 10.1016/j.jim.2011.12.001
M3 - Artículo
C2 - 22178422
AN - SCOPUS:84856527545
SN - 0022-1759
VL - 376
SP - 89
EP - 96
JO - Journal of Immunological Methods
JF - Journal of Immunological Methods
IS - 1-2
ER -