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Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients

Understanding the immunological phenotype of transplant recipients is important to improve outcomes and develop new therapies. Immunophenotyping of whole peripheral blood (WPB) by flow cytometry is a rapid method to obtain large amounts of data relating to the outcomes of different transplant treatm...

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Autores principales: Jimenez Vera, Elvira, Chew, Yi Vee, Nicholson, Leigh, Burns, Heather, Anderson, Patricia, Chen, Hsiao-Ting, Williams, Lindy, Keung, Karen, Zanjani, Negar Talaei, Dervish, Suat, Patrick, Ellis, Wang, Xin Maggie, Yi, Shounan, Hawthorne, Wayne, Alexander, Stephen, O’Connell, Philip J., Hu, Min
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6530858/
https://www.ncbi.nlm.nih.gov/pubmed/31116766
http://dx.doi.org/10.1371/journal.pone.0217163
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author Jimenez Vera, Elvira
Chew, Yi Vee
Nicholson, Leigh
Burns, Heather
Anderson, Patricia
Chen, Hsiao-Ting
Williams, Lindy
Keung, Karen
Zanjani, Negar Talaei
Dervish, Suat
Patrick, Ellis
Wang, Xin Maggie
Yi, Shounan
Hawthorne, Wayne
Alexander, Stephen
O’Connell, Philip J.
Hu, Min
author_facet Jimenez Vera, Elvira
Chew, Yi Vee
Nicholson, Leigh
Burns, Heather
Anderson, Patricia
Chen, Hsiao-Ting
Williams, Lindy
Keung, Karen
Zanjani, Negar Talaei
Dervish, Suat
Patrick, Ellis
Wang, Xin Maggie
Yi, Shounan
Hawthorne, Wayne
Alexander, Stephen
O’Connell, Philip J.
Hu, Min
author_sort Jimenez Vera, Elvira
collection PubMed
description Understanding the immunological phenotype of transplant recipients is important to improve outcomes and develop new therapies. Immunophenotyping of whole peripheral blood (WPB) by flow cytometry is a rapid method to obtain large amounts of data relating to the outcomes of different transplant treatments with limited patient impact. Healthy individuals and patients with type 1 diabetes (T1D) enrolled in islet transplantation were recruited and WPB was collected. 46 fluorochrome-conjugated mouse-anti-human antibodies were used (43 of 46 antibodies were titrated). BD cytometer setup and tracking beads were used to characterize and adjust for cytometer performance. Antibody cocktails were pre-mixed <60 minutes before staining. Multicolour panels were designed based on fluorochrome brightness, antigen density, co-expression, and fluorochrome spillover into non-primary detectors in each panel on a 5 laser flow cytometer. WPB sample staining used 50–300 μl WPB for each panel and was performed within 2 hours of blood sample collection. Samples were acquired on a BD-LSRFortessa. The operating procedures, including specimen collection, antibody cocktails, staining protocol, flow-cytometer setup and data analysis, were standardized. The staining index of 43 antibodies and the spillover spreading matrix for each panel was calculated. The final concentrations for the 46 antibodies used was determined for staining of WPB samples. Absolute cell-count and 7 leukocyte profiling panels consisting of subsets and/or status of granulocytes, monocytes, dendritic, B, NK, and T cells including regulatory T cells (Tregs) and NKT were designed and established on a 5 laser BD-LSR Fortessa. 13 T1D patients, including 4 islet transplant recipients and 8 healthy controls, were evaluated. The ability to reproducibly measure immune subsets and immune-profiles of islet transplant patients up to 18 months post transplantation has been established as a tool to measure immune cell reconstitution after transplantation.
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spelling pubmed-65308582019-05-31 Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients Jimenez Vera, Elvira Chew, Yi Vee Nicholson, Leigh Burns, Heather Anderson, Patricia Chen, Hsiao-Ting Williams, Lindy Keung, Karen Zanjani, Negar Talaei Dervish, Suat Patrick, Ellis Wang, Xin Maggie Yi, Shounan Hawthorne, Wayne Alexander, Stephen O’Connell, Philip J. Hu, Min PLoS One Research Article Understanding the immunological phenotype of transplant recipients is important to improve outcomes and develop new therapies. Immunophenotyping of whole peripheral blood (WPB) by flow cytometry is a rapid method to obtain large amounts of data relating to the outcomes of different transplant treatments with limited patient impact. Healthy individuals and patients with type 1 diabetes (T1D) enrolled in islet transplantation were recruited and WPB was collected. 46 fluorochrome-conjugated mouse-anti-human antibodies were used (43 of 46 antibodies were titrated). BD cytometer setup and tracking beads were used to characterize and adjust for cytometer performance. Antibody cocktails were pre-mixed <60 minutes before staining. Multicolour panels were designed based on fluorochrome brightness, antigen density, co-expression, and fluorochrome spillover into non-primary detectors in each panel on a 5 laser flow cytometer. WPB sample staining used 50–300 μl WPB for each panel and was performed within 2 hours of blood sample collection. Samples were acquired on a BD-LSRFortessa. The operating procedures, including specimen collection, antibody cocktails, staining protocol, flow-cytometer setup and data analysis, were standardized. The staining index of 43 antibodies and the spillover spreading matrix for each panel was calculated. The final concentrations for the 46 antibodies used was determined for staining of WPB samples. Absolute cell-count and 7 leukocyte profiling panels consisting of subsets and/or status of granulocytes, monocytes, dendritic, B, NK, and T cells including regulatory T cells (Tregs) and NKT were designed and established on a 5 laser BD-LSR Fortessa. 13 T1D patients, including 4 islet transplant recipients and 8 healthy controls, were evaluated. The ability to reproducibly measure immune subsets and immune-profiles of islet transplant patients up to 18 months post transplantation has been established as a tool to measure immune cell reconstitution after transplantation. Public Library of Science 2019-05-22 /pmc/articles/PMC6530858/ /pubmed/31116766 http://dx.doi.org/10.1371/journal.pone.0217163 Text en © 2019 Jimenez Vera et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Jimenez Vera, Elvira
Chew, Yi Vee
Nicholson, Leigh
Burns, Heather
Anderson, Patricia
Chen, Hsiao-Ting
Williams, Lindy
Keung, Karen
Zanjani, Negar Talaei
Dervish, Suat
Patrick, Ellis
Wang, Xin Maggie
Yi, Shounan
Hawthorne, Wayne
Alexander, Stephen
O’Connell, Philip J.
Hu, Min
Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
title Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
title_full Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
title_fullStr Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
title_full_unstemmed Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
title_short Standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
title_sort standardisation of flow cytometry for whole blood immunophenotyping of islet transplant and transplant clinical trial recipients
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6530858/
https://www.ncbi.nlm.nih.gov/pubmed/31116766
http://dx.doi.org/10.1371/journal.pone.0217163
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