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Using genome editing to engineer universal platelets
Author(s) -
Moyra Lawrence,
Annett Mueller,
Cédric Ghevaert
Publication year - 2019
Publication title -
emerging topics in life sciences
Language(s) - English
Resource type - Journals
eISSN - 2397-8562
pISSN - 2397-8554
DOI - 10.1042/etls20180153
Subject(s) - genome editing , crispr , platelet , induced pluripotent stem cell , computational biology , biology , thrombopoiesis , genome , transcription activator like effector nuclease , cas9 , computer science , microbiology and biotechnology , megakaryocyte , stem cell , immunology , genetics , haematopoiesis , gene , embryonic stem cell
Genome editing technologies such as zinc finger nucleases, TALENs and CRISPR/Cas9 have recently emerged as tools with the potential to revolutionise cellular therapy. This is particularly exciting for the field of regenerative medicine, where the large-scale, quality-controlled editing of large numbers of cells could generate essential cellular products ready to move towards the clinic. This review details recent progress towards generating HLA Class I null platelets using genome editing technologies for β2-microglobulin deletion, generating a universally transfusable cellular product. In addition, we discuss various methods for megakaryocyte (MK) production from human pluripotent stem cells and subsequent platelet production from the MKs. As well as simply producing platelets, differentiating MK cultures can enable us to understand megakaryopoiesis in vivo and take steps towards ameliorating bleeding disorders or deficiencies in MK maturation in patients. Thus by intersecting both these areas of research, we can produce optimised differentiation systems for the production of universal platelets, thus offering a stable supply of platelets for difficult-to-match patients and providing areas with transmissible disease concerns or an unpredictable supply of platelets with a steady supply of quality-controlled platelet units.

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