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Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model

[Image: see text] Introduction: Measurement of pancreatic beta cell mass in animal models is a common assay in diabetes researches. Novel whole-organ clearance methods in conjunction with transgenic mouse models hold tremendous promise to improve beta cell mass measurement methods. Here, we proposed...

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Autores principales: Karami, Fatemeh, Asgari Abibeiglou, Behrouz, Pahlavanneshan, Saghar, Farrokhi, Ali, Tamadon, Amin, Basiri, Mohsen, Khalooghi, Keynoosh, Fallahi, Majid, Tahamtani, Yaser
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Tabriz University of Medical Sciences (TUOMS Publishing Group) 2022
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9596880/
https://www.ncbi.nlm.nih.gov/pubmed/36381631
http://dx.doi.org/10.34172/bi.2022.23840
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author Karami, Fatemeh
Asgari Abibeiglou, Behrouz
Pahlavanneshan, Saghar
Farrokhi, Ali
Tamadon, Amin
Basiri, Mohsen
Khalooghi, Keynoosh
Fallahi, Majid
Tahamtani, Yaser
author_facet Karami, Fatemeh
Asgari Abibeiglou, Behrouz
Pahlavanneshan, Saghar
Farrokhi, Ali
Tamadon, Amin
Basiri, Mohsen
Khalooghi, Keynoosh
Fallahi, Majid
Tahamtani, Yaser
author_sort Karami, Fatemeh
collection PubMed
description [Image: see text] Introduction: Measurement of pancreatic beta cell mass in animal models is a common assay in diabetes researches. Novel whole-organ clearance methods in conjunction with transgenic mouse models hold tremendous promise to improve beta cell mass measurement methods. Here, we proposed a refined method to estimate the beta cell mass using a new transgenic Tg(Pdx1-GFP) mouse model and a recently developed free-of-acrylamide clearing tissue (FACT) protocol. Methods: First, we generated and evaluated a Tg(Pdx1-GFP) transgenic mouse model. Using the FACT protocol in our model, we could quantify the beta cell mass and alloxan-induced beta cell destruction in whole pancreas specimens. Results: Compiled fluorescent images of pancreas resulted in enhanced beta cell mass characterization in FACT-cleared sections (2928869±120215 AU) compared to No-FACT cleared sections (1292372±325632 AU). Additionally, the total number of detected islets with this method was significantly higher than the other clearance methods (155.7 and 109, respectively). Using this method, we showed green fluorescent protein (GFP) expression confined to beta cells in Tg(Pdx1-GFP) transgenic. This enhanced GFP expression enabled us to accurately measure beta cell loss in a beta cell destruction model. The results suggest that our proposed method can be used as a simple, and rapid assay for beta cell mass measurement in islet biology and diabetes studies. Conclusion: The Tg(Pdx1-GFP) transgenic mouse in conjunction with the FACT protocol can enhance large-scale screening studies in the field of diabetes.
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spelling pubmed-95968802022-11-14 Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model Karami, Fatemeh Asgari Abibeiglou, Behrouz Pahlavanneshan, Saghar Farrokhi, Ali Tamadon, Amin Basiri, Mohsen Khalooghi, Keynoosh Fallahi, Majid Tahamtani, Yaser Bioimpacts Original Research [Image: see text] Introduction: Measurement of pancreatic beta cell mass in animal models is a common assay in diabetes researches. Novel whole-organ clearance methods in conjunction with transgenic mouse models hold tremendous promise to improve beta cell mass measurement methods. Here, we proposed a refined method to estimate the beta cell mass using a new transgenic Tg(Pdx1-GFP) mouse model and a recently developed free-of-acrylamide clearing tissue (FACT) protocol. Methods: First, we generated and evaluated a Tg(Pdx1-GFP) transgenic mouse model. Using the FACT protocol in our model, we could quantify the beta cell mass and alloxan-induced beta cell destruction in whole pancreas specimens. Results: Compiled fluorescent images of pancreas resulted in enhanced beta cell mass characterization in FACT-cleared sections (2928869±120215 AU) compared to No-FACT cleared sections (1292372±325632 AU). Additionally, the total number of detected islets with this method was significantly higher than the other clearance methods (155.7 and 109, respectively). Using this method, we showed green fluorescent protein (GFP) expression confined to beta cells in Tg(Pdx1-GFP) transgenic. This enhanced GFP expression enabled us to accurately measure beta cell loss in a beta cell destruction model. The results suggest that our proposed method can be used as a simple, and rapid assay for beta cell mass measurement in islet biology and diabetes studies. Conclusion: The Tg(Pdx1-GFP) transgenic mouse in conjunction with the FACT protocol can enhance large-scale screening studies in the field of diabetes. Tabriz University of Medical Sciences (TUOMS Publishing Group) 2022 2022-05-28 /pmc/articles/PMC9596880/ /pubmed/36381631 http://dx.doi.org/10.34172/bi.2022.23840 Text en © 2022 The Author(s). https://creativecommons.org/licenses/by-nc/4.0/ This work is published by BioImpacts as an open access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/4.0/ (https://creativecommons.org/licenses/by-nc/4.0/) ). Non-commercial uses of the work are permitted, provided the original work is properly cited.
spellingShingle Original Research
Karami, Fatemeh
Asgari Abibeiglou, Behrouz
Pahlavanneshan, Saghar
Farrokhi, Ali
Tamadon, Amin
Basiri, Mohsen
Khalooghi, Keynoosh
Fallahi, Majid
Tahamtani, Yaser
Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model
title Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model
title_full Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model
title_fullStr Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model
title_full_unstemmed Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model
title_short Enhanced characterization of beta cell mass in a Tg(Pdx1-GFP) mouse model
title_sort enhanced characterization of beta cell mass in a tg(pdx1-gfp) mouse model
topic Original Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9596880/
https://www.ncbi.nlm.nih.gov/pubmed/36381631
http://dx.doi.org/10.34172/bi.2022.23840
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