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1
Valérie Deffontaine
08/06/2017
Characterisation of human
pluripotent stem cells (ESC & IPSC)
and by-products
2
Summary
1. Introduction: ESC and IPSC in the cell therapy area
2. Focus on the analytics and characterisation methods
3. Characterisation of ESC/IPSC and by-products (MSC
and cardiomyocytes like cells)
4. We know…we share: observations from our analytical
experiments
3
ESC and IPSC in the cell therapy area
EMBRYONICSTEMCELLSINDUCEDPLURIPOTENT
STEMCELLS
Skin Fibroblasts
Blastocyst
4
ESC and IPSC in the cell therapy area
DIFFERENTIATION
CELL-BASED THERAPY
AUTOLOGOUS ALLOGENIC
5
ESC and IPSC in the cell therapy area
Modified from Bionest Partners, 2010
Personalised cell
therapyDisease modelling
Drug discovery
Safety pharmacology
11 years after the discovery of IPSC…the goal has shifted!
6
ESC and IPSC in the cell therapy area
Adapted from Bionest Partners, 2010
7
ESC and IPSC in the cell therapy area
« IPS cells are only 10 years old. The research takes time. That’s
what everybody needs to understand » Shinya Yamanaka, Nobel
Prize Physiology Medicine 2012.
« The greatest future challenges are not scientific. Researchers are
going to need strong support from the pharmaceutical industry »
Edward Stevens, Pfizer Neuroscience and Pain Research Unit, UK.
Manufacturing Analytical
Services
8
Analytics and characterisation methods
Some definitions …
Analytics: science that seeks to the improvements of
substances (e.g. chemical) or entities (e.g. cell)
composition measurements and corresponding data
interpretation.
Validation: demonstrates that a method will provide
accurate, precise and reproductible data during the
study-sample analysis.
9
Analytics and characterisation methods
Selection of
validation
parameters
(validation or
qualification?)
Validation/
qualification
Pre-
validation/
qualification
System
Suitability
Tests
Development phase
10
Analytics and characterisation methods
CELL CHARACTERISATION
Identity
Purity/Impurities
Biological activity
(potency)
Viability
Mass
spectrometry
Microscopy
ELISA
Cell-based
assays
PCR
FACS
Microarrays
ECL
(MSD)
Luminex
11
Analytics and characterisation methods
CELL CHARACTERISATION
Identity
Purity/Impurities
Microscopy
PCR
FACS
12
ESC/IPSC characterisation
IPSC
ESI-017 Human Embryonic Stem Cells line (ESI BIO)
Human IPS Cells line (Applied StemCell)
ESC
13
ESC/IPSC characterisation
Method
Parameters
per sample
21 CFR part
11 compliant
software
Quantity of
cells per test
Time per
run
(analytics
+ process)
Flow
Cytometry
Quantitative +++ Yes Medium 2 days
QPCR
Semi
quantitative
++ Yes Small 1 day
Leica
Microscope
Mostly
qualitative
+ No High 3 to 4 days
BD FACSVerse™ &
FACSSuite™ software
Applied Biosystem™ 7500 Fast Real-
Time PCR & AccuSEQ™ software
Leica DMI6000B & Leica
Application Suites software
14
ESC/IPSC characterisation
Validation versus
Qualification
Reference material
Qualified cell bank
(marker expression
= 100%)
15
ESC/IPSC characterisation
Flow cytometry
TRA-1-60
SSEA-4
ALP
Rationale for the pluripotency panels design (Human)
SSEA-1
CD13
Sox2
Nanog
Oct3/4
Extracellular Intracellular
ESC/IPSC + ESC/IPSC - Original tissue
16
ESC/IPSC characterisation
Flow cytometry
Validation workflow (Positive markers)
16
ES/IPS cell banks
Labelling + Washing
ES/IPS ES/IPS
0.5*106c/ml
Accuracy, linearity (spikes, independant preparations)
1*106c/ml
0.5*106c/ml
Labelling plate
With antibodies cocktail
Without antibodies
cocktail
Analytical plate
17
ESC/IPSC characterisation
Flow cytometry
Validation workflow (Negative markers)
17
Positive cell line
banks
Labelling + Washing
Positive
cell line
0.5*106c/ml
Accuracy, linearity (spikes, independant preparations)
1*106c/ml
0.5*106c/ml
Labelling plate
With antibodies cocktail
Without antibodies
cocktail
Analytical plate
Positive
cell line
18
ESC/IPSC characterisation
Flow cytometry
Validation of intracellular panel on ESC
Spike 50:
50% labelled and 50%
unlabelled cells
45.83 % 47.24 % 47.30 %
Nanog Oct3/4 Sox2
Nanog Oct3/4 Sox2
19
ESC/IPSC characterisation
Flow cytometry
Validation of intracellular panel on ESC: linearity
20
ESC/IPSC characterisation
Flow cytometry
Validation of intra panel on ESC: accuracy
Nanog Oct3/4 Sox2
21
ESC/IPSC characterisation
Flow cytometry
Results: ESC & extracellular panel
98.96 %79.22 % 99.88 %0.05 %0.01 %
SSEA-1 CD13 TRA-1-60 SSEA-4 ALP
SSEA-1 CD13 TRA-1-60 SSEA-4 ALP
22
ESC/IPSC characterisation
Flow cytometry
Results: ESC & intracellular panel
99.12 % 99.49 % 99.95 %
Nanog Oct3/4 Sox2
Nanog Oct3/4 Sox2
23
ESC/IPSC characterisation
Flow cytometry
Results: IPSC & extracellular panel
98.12 % 91.20 %94.25 %0.05 %10.20 %
SSEA-1 CD13 TRA-1-60 SSEA-4 ALP
SSEA-1 CD13 TRA-1-60 SSEA-4 ALP
24
ESC/IPSC characterisation
Flow cytometry
Results: IPSC & intracellular panel
95.75 % 97.15 % 99.72 %
Nanog Oct3/4 Sox2
Nanog Oct3/4 Sox2
25
IPSC by-products characterisation
Study 1: Differentiation of IPSC in MSC-like cells
Step 1: Cells plating on 0.1% gelatin coated dishes in mTeSR 1 medium.
Step 2: Derivation step in 50% mTeSR 1 and 50 % derivation medium (alpha MEM,10% FBS,50 µM
magnesium L-ascrobic acid,100 nM dexamethasone).
Step 3: Derivation step in 100% derivation medium.
Step 4: Expansion step in expansion medium (20% O2) (Alpha MEM,10% heat inactivated FBS,1X
non essential amino acid,200 mM L-glutamine) or CellGro medium + FGF2 (3% O2).
26
IPSC by-products characterisation
Flow cytometry
CD44
CD90
CD105
CD45
MSC (Extracellular) IPSC (Extracellular)
Pos Markers Neg Markers
Differentiation of IPSC in MSC-like cells
CD34
ALP
EpCam
TRA-1-60
SSEA-1
27
ESC/IPSC: by-products characterisation
Flow cytometry
Differentiation of IPSC in MSC-like cells
Trend
28
ESC/IPSC: by-products characterisation
Flow cytometry
Differentiation of IPSC in MSC-like cells
Trend
29
ESC/IPSC: by-products characterisation
Flow cytometry
Differentiation of IPSC in MSC-like cells
Trend
30
ESC/IPSC: by-products characterisation
Flow cytometry
Differentiation of IPSC in MSC-like cells
Trend
31
IPSC by-products characterisation
Ventricular cardiomyocytes
(Cor.4U®)
Study 2: IPSC-derived cardiomyocytes (Axiogenesis)
Ventricular, atrial and
pacemaker cardiomyocytes
(CorV.4U®)
Cardiac fibroblasts
(FibroCor.4U®)
32
IPSC by-products characterisation
Flow cytometry
Pluripotency
(Extracellular)
Pluripotency
(Intracellular)
Identity
Impurities detection
IPSC-derived cardiomyocytes
TRA-1-60
SSEA-4
ALP
SSEA-1
CD13
Sox2
Nanog
Oct3/4
Cardio
(Intracellular)
Troponin
Actinin
Myosin
33
iPSC by-products characterisation
Flow cytometry
Ventricular
cardiomyocytes
Ventricular, atrial
and pacemakers
cardiomyocytes
Cardiac fibroblasts
iPSC-derived cardiomyocytes: Identity of cardiac cells
Cor.4U
CorV.4U
FibroCor.4U
Actinin TroponinMyosin
34
IPSC by-products characterisation
Flow cytometry
Individual
screening of 8
markers
iPSC-derived cardiomyocytes: Cell impurities in cardiomyocytes
35
IPSC by-products characterisation
Flow cytometry
Individual
screening of 8
markers
iPSC-derived cardiomyocytes: Cell impurities in cardiomyocytes
Multipotent cells? Pluripotent cells? Precursor cells?
36
IPSC by-products characterisation
Flow cytometry
Simultaneous
expression of
markers
Limit of Detection
(LOD)
iPSC-derived cardiomyocytes: Cell impurities in cardiomyocytes
Limit of Quantification
(LOQ)
37
IPSC by-products characterisation
QPCR
IPSC-derived cardiomyocytes: comparison of markers expression
Troponin
Myosin
Actinin
38
IPSC by-products characterisation
Microscopy
IPSC-derived cardiomyocytes
39
We know…we share:
Observations from our analytical experiments
Microscopy & QPCR
 Qualitative/Semi-quantitative methods
 Orthogonal methods for flow cytometry
 Microscopy: same antibody as for flow cytometry
but « pure »  availability !
 Supportive Data
40
We know…we share:
Observations from our analytical experiments
Flow cytometry
ESC and IPSC a story a little bit different…
 Cells growing in colonies
 Spontaneous differentiation
 Problem of viability, cell recovery for some cell lines,…
41
We know…we share:
Observations from our analytical experiments
Flow cytometry
SATISFACTORYFor identity testing
≥ 96 % ≥ 97 % 100 %
IPSC/ESC
≥ 93 % ≥ 95 % ≥ 96 %
IPSC derived
cardiomyocytes
Nanog Oct3/4 Sox2
Actinin Myosin Troponin
42
We know…we share:
Observations from our analytical experiments
Flow cytometry
QUESTIONABLEFor impurities detection
Autofluorescence
LOQ (~0.22 %) ?
43
Conclusions
PCR
 QPCR and microscopy: supportive data
 Flow cytometry: quantitative approach for identity tests
 Impurities detection: need for a new concept of test
44
Conclusions
PCR
 QPCR and microscopy: supportive data
 Flow cytometry: quantitative approach for identity tests
 Impurities detection: need for a new concept of test
What is the next analytical step for cell manufacturing?
Chaparro & Linero. 2016. Advanced Techniques
in Bone Regeneration. Chapter 12.
45
ACKNOWLEDGEMENTS
45
Arnaud DELOBEL
Nathalie DRAUX
Estelle LARA
Capucine LEPERS
Tristan PRITCHARD-MEAKER
Nicolas THEYS
Sandra THYS
Marie TOUSSAINT
Fabian VANDERMEERS
Kassandra WATILLON
46
valerie.deffontaine@quality-assistance.be
+32 71 53 47 81
www.quality-assistance.com
Technoparc de Thudinie, 2
B-6536 Donstiennes (Belgium)
Thank you for your attention
Any question?

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WEBINAR Characterisation of human pluripotent stem cells (ESCs and IPSC) and by-products

Editor's Notes

  1. The webinar of today will focus on the characterisation of cell-based medicinal products generated from embryonic stem cells and induced pluripotent stem cells culture. I will start my presentation with a brief introduction on the place of ESC and IPSC in the cell therapy area. Then I will focus my presentation on the methods to characterise these cells and their by products especially on the importance of the analytical work of method validation. Then I will present to you raw data coming from our projects of ESC and IPSC characterisations. Finally I will discuss these results and proposed some analytical recommendations.
  2. The ESC and IPSC are both pluripotent stem cells meaning that they can give rise to cell type from the three embyronic tissue: the mesoderm, endoderm and ectoderm. But the two cell types are not obtained by the same way in vitro. The starting material for an ESC culture is the inner cell mass of a blastocyst at day