Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells

Deficits in neuronal structure are consistently associated with neurodevelopmental illnesses such as autism and schizophrenia. Nonetheless, the inability to access neurons from clinical patients has limited the study of early neurostructural changes directly in patients’ cells. This obstacle has bee...

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Autores principales: Bellon, Alfredo, Hasoglu, Tuna, Peterson, Mallory, Gao, Katherine, Chen, Michael, Blandin, Elisabeta, Cortez-Resendiz, Alonso, Clawson, Gary A., Hong, Liyi Elliot
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2021
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Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8615477/
https://www.ncbi.nlm.nih.gov/pubmed/34827371
http://dx.doi.org/10.3390/brainsci11111372
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author Bellon, Alfredo
Hasoglu, Tuna
Peterson, Mallory
Gao, Katherine
Chen, Michael
Blandin, Elisabeta
Cortez-Resendiz, Alonso
Clawson, Gary A.
Hong, Liyi Elliot
author_facet Bellon, Alfredo
Hasoglu, Tuna
Peterson, Mallory
Gao, Katherine
Chen, Michael
Blandin, Elisabeta
Cortez-Resendiz, Alonso
Clawson, Gary A.
Hong, Liyi Elliot
author_sort Bellon, Alfredo
collection PubMed
description Deficits in neuronal structure are consistently associated with neurodevelopmental illnesses such as autism and schizophrenia. Nonetheless, the inability to access neurons from clinical patients has limited the study of early neurostructural changes directly in patients’ cells. This obstacle has been circumvented by differentiating stem cells into neurons, although the most used methodologies are time consuming. Therefore, we recently developed a relatively rapid (~20 days) protocol for transdifferentiating human circulating monocytes into neuronal-like cells. These monocyte-derived-neuronal-like cells (MDNCs) express several genes and proteins considered neuronal markers, such as MAP-2 and PSD-95. In addition, these cells conduct electrical activity. We have also previously shown that the structure of MDNCs is comparable with that of human developing neurons (HDNs) after 5 days in culture. Moreover, the neurostructure of MDNCs responds similarly to that of HDNs when exposed to colchicine and dopamine. In this manuscript, we expanded our characterization of MDNCs to include the expression of 12 neuronal genes, including tau. Following, we compared three different tracing approaches (two semi-automated and one automated) that enable tracing using photographs of live cells. This comparison is imperative for determining which neurite tracing method is more efficient in extracting neurostructural data from MDNCs and thus allowing researchers to take advantage of the faster yield provided by these neuronal-like cells. Surprisingly, it was one of the semi-automated methods that was the fastest, consisting of tracing only the longest primary and the longest secondary neurite. This tracing technique also detected more structural deficits. The only automated method tested, Volocity, detected MDNCs but failed to trace the entire neuritic length. Other advantages and disadvantages of the three tracing approaches are also presented and discussed.
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spelling pubmed-86154772021-11-26 Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells Bellon, Alfredo Hasoglu, Tuna Peterson, Mallory Gao, Katherine Chen, Michael Blandin, Elisabeta Cortez-Resendiz, Alonso Clawson, Gary A. Hong, Liyi Elliot Brain Sci Article Deficits in neuronal structure are consistently associated with neurodevelopmental illnesses such as autism and schizophrenia. Nonetheless, the inability to access neurons from clinical patients has limited the study of early neurostructural changes directly in patients’ cells. This obstacle has been circumvented by differentiating stem cells into neurons, although the most used methodologies are time consuming. Therefore, we recently developed a relatively rapid (~20 days) protocol for transdifferentiating human circulating monocytes into neuronal-like cells. These monocyte-derived-neuronal-like cells (MDNCs) express several genes and proteins considered neuronal markers, such as MAP-2 and PSD-95. In addition, these cells conduct electrical activity. We have also previously shown that the structure of MDNCs is comparable with that of human developing neurons (HDNs) after 5 days in culture. Moreover, the neurostructure of MDNCs responds similarly to that of HDNs when exposed to colchicine and dopamine. In this manuscript, we expanded our characterization of MDNCs to include the expression of 12 neuronal genes, including tau. Following, we compared three different tracing approaches (two semi-automated and one automated) that enable tracing using photographs of live cells. This comparison is imperative for determining which neurite tracing method is more efficient in extracting neurostructural data from MDNCs and thus allowing researchers to take advantage of the faster yield provided by these neuronal-like cells. Surprisingly, it was one of the semi-automated methods that was the fastest, consisting of tracing only the longest primary and the longest secondary neurite. This tracing technique also detected more structural deficits. The only automated method tested, Volocity, detected MDNCs but failed to trace the entire neuritic length. Other advantages and disadvantages of the three tracing approaches are also presented and discussed. MDPI 2021-10-20 /pmc/articles/PMC8615477/ /pubmed/34827371 http://dx.doi.org/10.3390/brainsci11111372 Text en © 2021 by the authors. https://creativecommons.org/licenses/by/4.0/Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Bellon, Alfredo
Hasoglu, Tuna
Peterson, Mallory
Gao, Katherine
Chen, Michael
Blandin, Elisabeta
Cortez-Resendiz, Alonso
Clawson, Gary A.
Hong, Liyi Elliot
Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells
title Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells
title_full Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells
title_fullStr Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells
title_full_unstemmed Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells
title_short Optimization of Neurite Tracing and Further Characterization of Human Monocyte-Derived-Neuronal-like Cells
title_sort optimization of neurite tracing and further characterization of human monocyte-derived-neuronal-like cells
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8615477/
https://www.ncbi.nlm.nih.gov/pubmed/34827371
http://dx.doi.org/10.3390/brainsci11111372
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