Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing

Regular blood transfusion is the cornerstone of care for patients with red blood cell (RBC) disorders such as thalassaemia or sickle‐cell disease. With repeated transfusion, alloimmunisation often occurs due to incompatibility at the level of minor blood group antigens. We use CRISPR‐mediated genome...

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Autores principales: Hawksworth, Joseph, Satchwell, Timothy J, Meinders, Marjolein, Daniels, Deborah E, Regan, Fiona, Thornton, Nicole M, Wilson, Marieangela C, Dobbe, Johannes GG, Streekstra, Geert J, Trakarnsanga, Kongtana, Heesom, Kate J, Anstee, David J, Frayne, Jan, Toye, Ashley M
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley and Sons Inc. 2018
Materias:
Report
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5991592/
https://www.ncbi.nlm.nih.gov/pubmed/29700043
http://dx.doi.org/10.15252/emmm.201708454
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author Hawksworth, Joseph
Satchwell, Timothy J
Meinders, Marjolein
Daniels, Deborah E
Regan, Fiona
Thornton, Nicole M
Wilson, Marieangela C
Dobbe, Johannes GG
Streekstra, Geert J
Trakarnsanga, Kongtana
Heesom, Kate J
Anstee, David J
Frayne, Jan
Toye, Ashley M
author_facet Hawksworth, Joseph
Satchwell, Timothy J
Meinders, Marjolein
Daniels, Deborah E
Regan, Fiona
Thornton, Nicole M
Wilson, Marieangela C
Dobbe, Johannes GG
Streekstra, Geert J
Trakarnsanga, Kongtana
Heesom, Kate J
Anstee, David J
Frayne, Jan
Toye, Ashley M
author_sort Hawksworth, Joseph
collection PubMed
description Regular blood transfusion is the cornerstone of care for patients with red blood cell (RBC) disorders such as thalassaemia or sickle‐cell disease. With repeated transfusion, alloimmunisation often occurs due to incompatibility at the level of minor blood group antigens. We use CRISPR‐mediated genome editing of an immortalised human erythroblast cell line (BEL‐A) to generate multiple enucleation competent cell lines deficient in individual blood groups. Edits are combined to generate a single cell line deficient in multiple antigens responsible for the most common transfusion incompatibilities: ABO (Bombay phenotype), Rh (Rh(null)), Kell (K (0)), Duffy (Fy(null)), GPB (S−s−U−). These cells can be differentiated to generate deformable reticulocytes, illustrating the capacity for coexistence of multiple rare blood group antigen null phenotypes. This study provides the first proof‐of‐principle demonstration of combinatorial CRISPR‐mediated blood group gene editing to generate customisable or multi‐compatible RBCs for diagnostic reagents or recipients with complicated matching requirements.
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spelling pubmed-59915922018-06-20 Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing Hawksworth, Joseph Satchwell, Timothy J Meinders, Marjolein Daniels, Deborah E Regan, Fiona Thornton, Nicole M Wilson, Marieangela C Dobbe, Johannes GG Streekstra, Geert J Trakarnsanga, Kongtana Heesom, Kate J Anstee, David J Frayne, Jan Toye, Ashley M EMBO Mol Med Report Regular blood transfusion is the cornerstone of care for patients with red blood cell (RBC) disorders such as thalassaemia or sickle‐cell disease. With repeated transfusion, alloimmunisation often occurs due to incompatibility at the level of minor blood group antigens. We use CRISPR‐mediated genome editing of an immortalised human erythroblast cell line (BEL‐A) to generate multiple enucleation competent cell lines deficient in individual blood groups. Edits are combined to generate a single cell line deficient in multiple antigens responsible for the most common transfusion incompatibilities: ABO (Bombay phenotype), Rh (Rh(null)), Kell (K (0)), Duffy (Fy(null)), GPB (S−s−U−). These cells can be differentiated to generate deformable reticulocytes, illustrating the capacity for coexistence of multiple rare blood group antigen null phenotypes. This study provides the first proof‐of‐principle demonstration of combinatorial CRISPR‐mediated blood group gene editing to generate customisable or multi‐compatible RBCs for diagnostic reagents or recipients with complicated matching requirements. John Wiley and Sons Inc. 2018-04-26 2018-06 /pmc/articles/PMC5991592/ /pubmed/29700043 http://dx.doi.org/10.15252/emmm.201708454 Text en © 2018 The Authors. Published under the terms of the CC BY 4.0 license This is an open access article under the terms of the http://creativecommons.org/licenses/by/4.0/ License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.
spellingShingle Report
Hawksworth, Joseph
Satchwell, Timothy J
Meinders, Marjolein
Daniels, Deborah E
Regan, Fiona
Thornton, Nicole M
Wilson, Marieangela C
Dobbe, Johannes GG
Streekstra, Geert J
Trakarnsanga, Kongtana
Heesom, Kate J
Anstee, David J
Frayne, Jan
Toye, Ashley M
Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing
title Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing
title_full Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing
title_fullStr Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing
title_full_unstemmed Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing
title_short Enhancement of red blood cell transfusion compatibility using CRISPR‐mediated erythroblast gene editing
title_sort enhancement of red blood cell transfusion compatibility using crispr‐mediated erythroblast gene editing
topic Report
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5991592/
https://www.ncbi.nlm.nih.gov/pubmed/29700043
http://dx.doi.org/10.15252/emmm.201708454
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