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CD34+ AND HUMAN INDUCED PLURIPOTENT STEM CELL (IPSC) DIFFERENTIATION TO TRANSFUSION READY RED BLOOD CELLS
Author(s):
Marie-José Claessen
,
Marie-José Claessen
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands;Hematology,AMC Amsterdam,Amsterdam,Netherlands
Eszter Varga
,
Eszter Varga
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Marten Hansen
,
Marten Hansen
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Patrick Burger
,
Patrick Burger
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Steven Heshusius
,
Steven Heshusius
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Tatjana Wust
,
Tatjana Wust
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Jesse Eernstman
,
Jesse Eernstman
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Marijke Thiel
,
Marijke Thiel
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Esther Heideveld
,
Esther Heideveld
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Erica Sellink
,
Erica Sellink
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Marieke von Lindern
,
Marieke von Lindern
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
Emile van den Akker
Emile van den Akker
Affiliations:
Hematopoiesis,Sanquin Research,Amsterdam,Netherlands
(Abstract release date: 05/18/17) EHA Library. Claessen M. 06/23/17; 181419; S132
Marie-Jose Claessen
Marie-Jose Claessen
Contributions
PDF Abstract
Abstract

Abstract: S132

Type: Oral Presentation

Presentation during EHA22: On Friday, June 23, 2017 from 12:30 - 12:45

Location: Room N105

Background

Donor-derived red blood cells (RBC) are the most common form of cellular therapy. However the source of cells is dependent on donor availability with a potential risk of allo-immunization and blood borne diseases.

Aims
We aim to produce unlimited numbers of cultured RBC with a defined `universal donor´ phenotype for transfusion purposes.

Methods
To this end we prepare for a clinical test using autologous cultured RBC to test their in vivo stability. In parallel we develop methods for unlimited production of cultured RBC. An immortal source to produce in vitro cultured RBCs (cRBC), such as iPSCs would allow selection of `universal donor` RBC, or  provide an autologous end product with the absence of immune reactions.

Results

The in vitro production of RBC has proven to be successful, however there are barriers to overcome prior to clinical application. e.g: xeno-free culturing methods, scale up cultures to obtain transfusion units (1-2*1012 erythrocytes), and for iPSC we need virus- and transgene-free reprogramming protocols.
To solve the above mentioned issues a customized humanized GMP-grade medium (Cellquin) was generated in order to control erythroid culture parameters and to reduce culture costs. This medium allowed 1*108 times erythroid expansion from PBMCs to pure adult EBL cultures within 25 days, comparable to non-GMP commercial media. To generate iPSC, a non-integrative polycistronic episomal vector containing (OCT4-SOX2-KLF4-cMYC-LIN28) was used to reprogram PBMC-expanded EBLs to iPSC, displaying pluripotency potential and normal karyotype. iPSCs were adapted to single cell passage allowing directed colony differentiation using a feeder-free monolayer approach. From day 6 of differentiation Cellquin was applied with lineage-specific growth factors, resulted iPSC differentiation to EBLs which was initiated by the appearance of hemogenic endothelium following hematopoietic specification. Our differentiation method resulted in ~150*106 CD41- CD34- CD71+ CD235+ CD36+ expanded EBLs from 1200 iPSCs within 21 days (12 days of iPSC diff. + 9 days of expansion). Further maturation of iPSC-EBLs yielded CD71+ CD235+ CD36- pure orthochromatic normoblasts expressing mainly gamma globin chains (fetal) and small amount of beta globins (adult) in agreement with literature. Currently we are testing enucleation potential of matured iPSC-EBLs.

Conclusion

Here we showed that our monolayer approach is simple, highly controlled and compatible with upscaling. Avoiding virus-, integrative reprogramming, feeders and with our GMP-grade media we maintained a cost effective system moving toward clinical application.

Session topic: 30. Transfusion medicine

Keyword(s): transfusion, Erythroid differentiation, Erythroid cells, ABO blood group

Abstract: S132

Type: Oral Presentation

Presentation during EHA22: On Friday, June 23, 2017 from 12:30 - 12:45

Location: Room N105

Background

Donor-derived red blood cells (RBC) are the most common form of cellular therapy. However the source of cells is dependent on donor availability with a potential risk of allo-immunization and blood borne diseases.

Aims
We aim to produce unlimited numbers of cultured RBC with a defined `universal donor´ phenotype for transfusion purposes.

Methods
To this end we prepare for a clinical test using autologous cultured RBC to test their in vivo stability. In parallel we develop methods for unlimited production of cultured RBC. An immortal source to produce in vitro cultured RBCs (cRBC), such as iPSCs would allow selection of `universal donor` RBC, or  provide an autologous end product with the absence of immune reactions.

Results

The in vitro production of RBC has proven to be successful, however there are barriers to overcome prior to clinical application. e.g: xeno-free culturing methods, scale up cultures to obtain transfusion units (1-2*1012 erythrocytes), and for iPSC we need virus- and transgene-free reprogramming protocols.
To solve the above mentioned issues a customized humanized GMP-grade medium (Cellquin) was generated in order to control erythroid culture parameters and to reduce culture costs. This medium allowed 1*108 times erythroid expansion from PBMCs to pure adult EBL cultures within 25 days, comparable to non-GMP commercial media. To generate iPSC, a non-integrative polycistronic episomal vector containing (OCT4-SOX2-KLF4-cMYC-LIN28) was used to reprogram PBMC-expanded EBLs to iPSC, displaying pluripotency potential and normal karyotype. iPSCs were adapted to single cell passage allowing directed colony differentiation using a feeder-free monolayer approach. From day 6 of differentiation Cellquin was applied with lineage-specific growth factors, resulted iPSC differentiation to EBLs which was initiated by the appearance of hemogenic endothelium following hematopoietic specification. Our differentiation method resulted in ~150*106 CD41- CD34- CD71+ CD235+ CD36+ expanded EBLs from 1200 iPSCs within 21 days (12 days of iPSC diff. + 9 days of expansion). Further maturation of iPSC-EBLs yielded CD71+ CD235+ CD36- pure orthochromatic normoblasts expressing mainly gamma globin chains (fetal) and small amount of beta globins (adult) in agreement with literature. Currently we are testing enucleation potential of matured iPSC-EBLs.

Conclusion

Here we showed that our monolayer approach is simple, highly controlled and compatible with upscaling. Avoiding virus-, integrative reprogramming, feeders and with our GMP-grade media we maintained a cost effective system moving toward clinical application.

Session topic: 30. Transfusion medicine

Keyword(s): transfusion, Erythroid differentiation, Erythroid cells, ABO blood group

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