Cas9-AAV6 gene correction of beta-globin in autologous HSCs improves sickle cell disease erythropoiesis in mice.
Adam C WilkinsonDaniel P DeverRon BaikJoab CamarenaIan HsuCarsten T CharlesworthChika MoritaHiromitsu NakauchiMatthew H PorteusPublished in: Nature communications (2021)
CRISPR/Cas9-mediated beta-globin (HBB) gene correction of sickle cell disease (SCD) patient-derived hematopoietic stem cells (HSCs) in combination with autologous transplantation represents a recent paradigm in gene therapy. Although several Cas9-based HBB-correction approaches have been proposed, functional correction of in vivo erythropoiesis has not been investigated previously. Here, we use a humanized globin-cluster SCD mouse model to study Cas9-AAV6-mediated HBB-correction in functional HSCs within the context of autologous transplantation. We discover that long-term multipotent HSCs can be gene corrected ex vivo and stable hemoglobin-A production can be achieved in vivo from HBB-corrected HSCs following autologous transplantation. We observe a direct correlation between increased HBB-corrected myeloid chimerism and normalized in vivo red blood cell (RBC) features, but even low levels of chimerism resulted in robust hemoglobin-A levels. Moreover, this study offers a platform for gene editing of mouse HSCs for both basic and translational research.
Keyphrases
- sickle cell disease
- crispr cas
- red blood cell
- cell therapy
- genome editing
- gene therapy
- bone marrow
- stem cells
- copy number
- mouse model
- genome wide
- platelet rich plasma
- type diabetes
- skeletal muscle
- acute myeloid leukemia
- mesenchymal stem cells
- metabolic syndrome
- genome wide identification
- insulin resistance
- acute lymphoblastic leukemia
- high fat diet induced
- high resolution
- single cell
- wild type
- high speed