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A Universal System for Highly Efficient Cardiac Differentiation of Human Induced Pluripotent Stem Cells That Eliminates Interline Variability

Author: A Moretti
A Peters
Ann Peters
BE Reubinoff
C Allegrucci
C Denning
C Freund
C Mummery
C Xu
C Xu
C Xu
CS Chen
D Evseenko
E Bettiol
Elias T. Zambidis
EM Hansson
G Proetzel
H Gai
H Segev
H Skottman
HF Chen
I Itzhaki
I Kehat
I Kehat
IH Park
J Yu
J Zhang
JA Thomson
JC Moore
JM Polo
K Kim
K Osafune
L Warren
L Yang
Leslie Tung
M Barron
M Pekkanen-Mattila
MA Laflamme
Martin Pera
MC Marchetto
MC Simon
MD Ungrin
MH Chin
Michal A. Millrod
MV Pryzhkova
MV Wiles
O Adewumi
P Zhang
Paul W. Burridge
PW Burridge
R Passier
RI Freshney
S Kaichi
S Niebruegge
S Takei
S Weinberg
SA Jackson
Seth Weinberg
SL Paige
SR Braam
Susan Thompson
TH Tran
Vasiliki Mahairaki
Vassilis E. Koliatsos
WE Lowry
XQ Xu
Xuan Yuan
Publication venue: Public Library of Science
Publication date: 01/04/2011
Field of study

The production of cardiomyocytes from human induced pluripotent stem cells (hiPSC) holds great promise for patient-specific cardiotoxicity drug testing, disease modeling, and cardiac regeneration. However, existing protocols for the differentiation of hiPSC to the cardiac lineage are inefficient and highly variable. We describe a highly efficient system for differentiation of human embryonic stem cells (hESC) and hiPSC to the cardiac lineage. This system eliminated the variability in cardiac differentiation capacity of a variety of human pluripotent stem cells (hPSC), including hiPSC generated from CD34(+) cord blood using non-viral, non-integrating methods.We systematically and rigorously optimized >45 experimental variables to develop a universal cardiac differentiation system that produced contracting human embryoid bodies (hEB) with an improved efficiency of 94.7±2.4% in an accelerated nine days from four hESC and seven hiPSC lines tested, including hiPSC derived from neonatal CD34(+) cord blood and adult fibroblasts using non-integrating episomal plasmids. This cost-effective differentiation method employed forced aggregation hEB formation in a chemically defined medium, along with staged exposure to physiological (5%) oxygen, and optimized concentrations of mesodermal morphogens BMP4 and FGF2, polyvinyl alcohol, serum, and insulin. The contracting hEB derived using these methods were composed of high percentages (64-89%) of cardiac troponin I(+) cells that displayed ultrastructural properties of functional cardiomyocytes and uniform electrophysiological profiles responsive to cardioactive drugs.This efficient and cost-effective universal system for cardiac differentiation of hiPSC allows a potentially unlimited production of functional cardiomyocytes suitable for application to hPSC-based drug development, cardiac disease modeling, and the future generation of clinically-safe nonviral human cardiac cells for regenerative medicine

Public Library of Science (PLOS)

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