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Optimising methods for human thyroid primary cell culture isolation

Arenal, Valentina; Madsen, Clara; Fernández Chávez, LucíaIcon ; Alonso, Exequiel GonzaloIcon ; Pichel, Pamela; Recio, Sergio; Fermento, María EugeniaIcon ; Alonso, Eliana NoeliaIcon ; Ferronato, María JuliaIcon ; Facchinetti, Maria MartaIcon ; Curino, Alejandro CarlosIcon ; Colo, Georgina PamelaIcon
Tipo del evento: Mesa redonda
Nombre del evento: LXIX Reunión Anual De La Sociedad Argentina de Investigación Clínica; XXVI Sociedad Argentina De Fisiología y Asociación Latinoamericana De Ciencias Fisiológicas
Fecha del evento: 19/11/2024
Institución Organizadora: Sociedad Argentina De Investigación Clínica; Sociedad Argentina De Fisiología; Asociación Latinoamericana De Ciencias Fisiológicas;
Título de la revista: Medicina (Buenos Aires)
Editorial: Fundación Revista Medicina
ISSN: 1669-9106
Idioma: Inglés
Clasificación temática:
Bioquímica y Biología Molecular

Resumen

According to the GLOBOCAN 2020 database on cancer incidence and mortality, thyroid cancer (TC) has the ninth-highest cancer in- cidence worldwide. Basic research contributes to developing diag- nostic and treatment alternatives. Cell models play a crucial role in vitro study of the thyroid. Permanent thyroid cell lines widely used in laboratory research typically originate from tumors. However, there is a need to compare these tumor cells with cells originating from normal thyroid tissue. Primary cell lines are invaluable for exploring cancer biology and investigating novel treatments. This study aims is optimize an isolation protocol of human primary thyroid cells from histologically non-tumor, tumor, and metastasis tissues. Primary cul- tures are laborious to obtain and then difficult to maintain in culture. We tried five different methods for isolating primary cells that com- bine mechanical disaggregation and enzymatic digestion. These methods use distinct enzymatic compositions, incubation times, and mechanical approaches, including centrifugation. We have ar- rived at a simple, rapid, and effective method to culture cells from thyroid biopsies for subsequent studies. Our previous results have revealed that GEF-H1 plays a pro-tumor role in different tumoral cell lines. We investigate the expression of GEF-H1, which belongs to the RhoA-GTPase activator family, in primary cells. Using immu- nofluorescence staining, we observed significantly higher GEF-H1 protein expression in cytokeratin-19 positive thyroid carcinoma cells compared to normal thyroid cells (p<0.0001). Our results propose a cheap and easy isolation thyroid primary cells protocol and suggest that GEF-H1 could be used as a potential tumor biomarker in TC.
Palabras clave: THYROID CANCER , GEF-H1 , PRIMARY CELL CULTURE , METHODS
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info:eu-repo/semantics/openAccess Excepto donde se diga explícitamente, este item se publica bajo la siguiente descripción: Creative Commons Attribution-NonCommercial-ShareAlike 2.5 Unported (CC BY-NC-SA 2.5)
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URI: http://hdl.handle.net/11336/278852
URL: https://medicinabuenosaires.com/revistas/vol84-24/s5/1s5.pdf
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Eventos(INIBIBB)
Eventos de INST.DE INVEST.BIOQUIMICAS BAHIA BLANCA (I)
Citación
Optimising methods for human thyroid primary cell culture isolation; LXIX Reunión Anual De La Sociedad Argentina de Investigación Clínica; XXVI Sociedad Argentina De Fisiología y Asociación Latinoamericana De Ciencias Fisiológicas; Ciudad Autónoma de Buenos Aires; Argentina; 2024; 170-170
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