Research II Revised
Research II Revised
Research II Revised
Table of Contents
Title Page.........1
Table of Contents.....2
Acknowledgment.....3
Abstract....4
Chapter I The Problem and its Background..........5
Background of the Study.....5
Objectives....7
Significance of the Study....8
Scope and Limitation...8
Chapter II Conceptual Framework.......9
Definition of Terms.9
Related Literature and Studies...11
Chapter III Methodology17
Appropriateness of Research Design.17
Pilot Study.17
Research Setting18
Instrumentation..18
Procedure...19
Ethical Considerations...20
Chapter IV - Presentation, Analysis, And Interpretation...21
Chapter V - Summary of Findings, Conclusions, And Recommendations...36
Summary36
Conclusion.37
Recommendations..39
Bibliography..40
Appendices43
ACKNOWLEDGEMENT
This research is made possible through the help and support of everyone,
including our family, friends and faculties. We are grateful, first, to Our Lord for guiding
us and comforting us in finishing this research. We are also thankful to our instructor,
Engr. Jopeth Ramis, in supporting us, assisting us and imparting us his knowledge about
tissue engineering research.
We also expressed our gratitude to Chemical Engineering laboratory technicians
for their patience and for providing us laboratory apparatus we had used in the
experiment.
We are also thankful to the Lung Center of the Philippines and to UP Diliman
Chemical Engineering Department Laboratory for helping us and providing us apparatus
to obtain our results.
We are also grateful for the help of Safebirth Lying-in Clinic, East Avenue
Medical Center, and Dr. Jose Fabella Memorial Hospital for permitting us to get
placentas. Without them, this research was for nothing
Abstract
Tissue engineering has shown advancement in the medical field in recent years.
One of the most promising biological materials is human amniotic membrane which is
used as a scaffold for cell proliferation and differentiation. The HAM undergoes the
decellularization process, where cells are being removed so as to grow only the desirable
cells. The study aims to determine the most suitable combination of procedures for the
decellularization process. The amnions harvested and pretreated with 0.25, 0.5, 0.75and
1M NaClO or PBS was decellularized by either soaking or swabbing using 0.25, 0.5, 0.75
and 1M NaOH. Cell count results showed that the combination of 0.25 NaClO
pretreatment and 0.75M NaOH soaking of amnion was the best procedure because it
removed the most number of cells.
After a series of experimentations, the optimum process was determined to be the
soaking of amnion pretreated with 0.25 NaClO with 0.75M NaOH because of significant
effect in removing the cells and preserve the growth factors in amnions as based on the
FTIR results. Also this method is cost-effective, could save time and resources.
CHAPTER I
THE PROBLEM AND ITS BACKGROUND
the
scaffold
material
involves
the
decellularization
process.
Decellularization can be defined as the process of degrading the resident cells of a tissue
or an organ in order to derive the extracellular matrix of the primary tissue so that it can
be used as a scaffold material for the formation of the fabricated novel tissue.
These biologically derived matrices can come from various methods, such as
using chemical agents, enzymes, detergents, and physical and miscellaneous agents like
temperature, force, pressure, non-thermal irreversible electroporation. The effectiveness
of these agents is dependent on many factors including the tissue cellularity, density, lipid
content, and thickness. The removal agent has the possibility of producing undesirable
effects on the composition of the extracellular matrix and must also be considered [4].
The application of decellularization agents is characterized into four categories,
namely, whole organ perfusion, pressure gradient, supercritical fluid, immersion and
agitation. Each of these applications depends on the properties of the tissue and the
agents used. The choice of decellularization methods can be successful with a complete
General Objective
To produce a decellularized amnion tissue that is suited for creating a biologic
scaffold material.
1.2.2
Specific Objective
CHAPTER II
CONCEPTUAL FRAMEWORK
Decellularization Method
Rat liver
Porcine
liver
Mechanical perfusion
(electroporation)
Mouse heart
Porcine
trachea
Limitation
Disruption of
microfilament and
microtubule
Loss of cellmediated function
Disruption of
glycosaminoglycan,
reduce the laminin
and fibronectin
Various studies have been published to demonstrate the methodologies for whole
organ decellularization using different approaches but all have its limitations. These
includes Perfusion with detergents (SDS, Triton X-100); Mechanical perfusion
Amnion- a thin membrane that surrounds the fetus during pregnancy. The amnion is the
inner of the two fetal membranes and it contains the amniotic fluid.
Cell counting- cell counting is any of various methods for the counting or similar
quantification of cells in the life sciences, including medical diagnosis and treatment. It is
an important subset of cytometry, with applications in research and clinical practice.
Chorion- the outermost of the two fetal membranes that surround the embryo. The
chorion develops villi (vascular finger-like projections) and develops into the placenta.
Extracellular matrix (ECM) - substance produced by cells and secreted into the
environment in which the cells are embedded; contains collagen, proteoglycans,
glycosaminoglycans, and fluid; can influence the behavior of the cells.
Growth factor- any of a group of proteins that stimulate the growth of specific tissues.
Growth factors play an important role in promoting cellular differentiation and cell
division.
Placenta- A temporary organ that joins the mother and fetus, transferring oxygen and
nutrients from the mother to the fetus and permitting the release of carbon dioxide and
waste products from the fetus.
Swab- A wad of cotton, gauze, or other absorbent material attached to the end of a stick
or clamp, used to apply or remove a substance from a surface.
Trypan blue- is a vital stain used to selectively colour dead tissues or cells blue. It is a
diazo dye.
CHAPTER III
METHODOLOGY
Procedure
CHAPTER IV
In the present work, tissue decellularization was performed and confirmed prior to
use as scaffolds. Human amnion was harvested and decellularized and examined for cell
count and chemical composition before/after decellularization.
Figure 2. The graph shows the second derivative of the fresh amnion spectra which is in
transmission mode.
(b)
(d)
Table 1. Secondary derivative of FTIR spectra of (a) Raw Amnion (b) 0.25M (c) 0.50M (d) 1M
(Swabbed)
NaOH (Swabbed)
Fresh Amnion
Group Frequency
Wavenumber (cm-1)
3679-3577
3478-3329
3313-3236
3214-3135
2983-2892
2872-2810
1774-1702
1684-1588
1577-1496
1462-1417
1405-1337
1258-1185
Fresh Amnion
0.25M
0.50M
Peak
3620
3381
3264
3191
2928
2836
1738
1639
1536
1442
1369
1222
Functional Gro
3626-3581
3208-3079
3066-2928
2918-2844
1829-1678
1614-1565
1520-1459
3616
3149
3007
2890
1698
1596
1497
3634-3588
3230-3065
3065-2958
2236-2167
1845-1678
1611-1562
1536-1464
3615
3145
3017
2206
1706
1596
1505
3628-3586
3209-3060
3022-2970
1862-1678
1605-1529
3616
3132
3010
1706
1594
(a)
0.75M
3216-3087
3083-2949
1755-1684
1613-1559
1526-1455
1368-1326
1305-1264
1222-1155
3154
3008
1706
1597
1496
1363
1292
1199
Carboxylic Acids
Aromatics C-H
C=O
1 Amines N-H
Nitro Compounds
Alkanes C-H
Amine C-N
Amine C-N
1M
3216-3087
3083-2949
1755-1684
1613-1559
1526-1455
1368-1326
1305-1264
1222-1155
3154
3008
1706
1597
1496
1363
1292
1199
Carboxylic Acids
Aromatics C-H
C=O
1 Amines N-H
Nitro Compounds
Alkanes C-H
Amine C-N
Amine C-N
(c)
Table 2. Secondary derivative of FTIR spectra of (a) Raw Amnion (b) 0.25M (c) 0.50M (d) 1M
(Soaked)
Group Frequency
Wavenumber (cm-1)
Fresh Amnion
3679-3577
3478-3329
3313-3236
3214-3135
2983-2892
2872-2810
1774-1702
1684-1588
1577-1496
1462-1417
1405-1337
1258-1185
Fresh Amnion
0.25M
0.50M
Peak
3620
3381
3264
3191
2928
2836
1738
1639
1536
1442
1369
1222
Functional Grou
3626-3581
3208-3079
3066-2928
2918-2844
1829-1678
1614-1565
1520-1459
3616
3149
3007
2890
1698
1596
1497
3634-3588
3230-3065
3065-2958
2236-2167
1845-1678
1611-1562
1536-1464
3615
3145
3017
2206
1706
1596
1505
3628-3586
3209-3060
3022-2970
1862-1678
1605-1529
3616
3132
3010
1706
1594
3216-3087
3083-2949
1755-1684
1613-1559
1526-1455
1368-1326
1305-1264
1222-1155
3154
3008
1706
1597
1496
1363
1292
1199
Carboxylic Acids O
Aromatics C-H
C=O
1 Amines N-H
Nitro Compounds N
Alkanes C-H
Amine C-N
Amine C-N
1M
3216-3087
3083-2949
1755-1684
1613-1559
1526-1455
1368-1326
1305-1264
1222-1155
3154
3008
1706
1597
1496
1363
1292
1199
Carboxylic Acids O
Aromatics C-H
C=O
1 Amines N-H
Nitro Compounds N
Alkanes C-H
Amine C-N
Amine C-N
For the FTIR result of fresh amnion, organic compounds were identified from the
ranges of peaks observed from the graph. The graph reveals no IR bands in the triplebond region (25002000 cm1). Organic compounds from XH stretching region (4000
2500 cm1), the double-bond region (20001500 cm1) and the fingerprint region (1500
600 cm1) were determined. The fundamental vibrations in the 40002500 cm1 region
are generally due to OH, CH and NH stretching. The principal bands in the 2000
1500 cm1 region are due to C=C and C=O stretching. 12201020 cm1 is due to Aliphatic
CN stretching.
Comparing the graph of swabbed decellularized amnion using 0.25M NaOH,
some IR bands are missing, indicating the change in chemical composition of the tissue.
In the XH stretching region (40002500 cm1), 1, 2 Amines, Amides N-H and
Carboxylic Acids O-H are missing. All the IR bands in the fingerprint region (1500600
(1500600 cm1). Though, in the double-bond region (20001500 cm 1) all the IR bands
remained.
functional groups that turn up. Moreover, there is an another Nitro Compounds N-O
appeared in the double-bond region (20001500 cm1)
Evaluating the graph of fresh amnion and decellularized amnion soaked using 1M
NaOH, the results are almost the same. In the XH stretching region (40002500 cm1),
1, 2 Amines, Amides N-H is missing. Amine C-N in the fingerprint region (1500600
cm1) is not present. Nevertheless, in the double-bond region (20001500 cm 1) all the IR
bands remained.
Fresh amnion
Figure 3. Second derivative infrared spectrum of fresh amnion. The deconvolution was
carried out by PeakFit software.
Figure 4. Tabulated results of the cell counting for different amnions pretreated with (a) PhosphateBuffered Saline solution, (b) 0.25M NaClO solution, (c) 0.50M NaClO solution, and (d) 0.75M NaClO
Figure 4 above shows the number of cells retained in the amnion after various
decellularization processes. The blue asterisk at the top of each data bar indicates the
significant difference of the number of retained cells in that set of trial to the fresh
amnion sample while the black bar indicates the significant difference between the two
data bar under it. Significant difference is expressed in p-value. Comparison of the
figures show that the best process in terms of cells removed is the soaking of the amnion
in 0.75 molar sodium hydroxide pre-treated with 0.25 molar sodium chlorate having a pvalue of 0.0204. Amnions with the same pretreatment but swabbed instead with 0.75
molar NaOH showed also a significant decrease in the number of cell compared with
Recommendations
With the data gathered and interpreted, the researchers arrived at certain
recommendations. The amnion pretreated with
soaked for more than 10 minutes using 0.75M NaOH solution. This would ensure better
denuding of the amnion. For future researchers, they are encouraged to venture on lower
concentrations of alkaline solution to be used. Additional experimentations on the
potentials of amnion as a biomaterial must be performed, meanwhile the process that was
formulated by this experiment establishes to be effective in preserving the growth factors
in amnion. Lastly, products from this experiment may be used to produce electro-spun
nanofibers.
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Fig. 2: Ms. Remy Magbiray orienting the students about the basics of Aseptic Procedures.
Fig. 3: Students wearing their PPEs together with Engr. Jopeth Ramis demonstrating the
proper aseptic procedures for the experiment.
Fig. 8(a)
Fig. 8 (b)
Fig. 8
M of
Trypan
Fig.
9(a)
With
trypan
blue
Fig. 9 (b)
Without trypan blue
Fig. 9: (a) and
(b) Decellularize amnion membrane.