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Laminin-111 Peptides Conjugated to Fibrin Hydrogels Promote Formation of Lumen Containing Parotid Gland Cell Clusters Kihoon Nam, Joshua P Jones, Pedro Lei, Stelios T. Andreadis, and Olga Juliana Baker Biomacromolecules, Just Accepted Manuscript • DOI: 10.1021/acs.biomac.6b00588 • Publication Date (Web): 05 May 2016 Downloaded from http://pubs.acs.org on May 11, 2016
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Biomacromolecules
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Laminin-111 Peptides Conjugated to Fibrin
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Hydrogels Promote Formation of Lumen Containing
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Parotid Gland Cell Clusters
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Kihoon Nam1, Joshua P. Jones2, Pedro Lei3, Stelios T. Andreadis3, 4, 5 and Olga J. Baker1*
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School of Dentistry, 2Department of Bioengineering, The University of Utah, Salt Lake City,
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UT 84108, USA, 3Department of Chemical and Biological Engineering, 4Department of
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Biomedical Engineering, School of Engineering and Applied Sciences, 5Center of Bioinformatics
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and Life Sciences, University at Buffalo, The State University of New York, Buffalo, NY 14260,
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USA.
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ABSTRACT
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Previous studies showed that mouse submandibular gland cells form three-dimensional
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structures when grown on Laminin-111 gels. The use of Laminin-111 for tissue bioengineering is
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complicated due to its lack of purity. In contrast, the use of synthetic peptides derived from
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Laminin-111 is beneficial due to their high purity and easy manipulation. Two Laminin-111
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peptides have been identified for salivary cells: the A99 peptide corresponding to the α1 chain
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from Laminin-111 and the YIGSR peptide corresponding to the β1 chain from Laminin-111,
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which are important for cell adhesion and migration. We created three-dimensional salivary cell
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clusters using a modified fibrin hydrogel matrix containing immobilized Laminin-111 peptides.
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Results indicate that the YIGSR peptide improved morphology and lumen formation in rat
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parotid Par-C10 cells as compared to cells grown on unmodified fibrin hydrogel. Moreover, a
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combination of both peptides not only allowed the formation of functional three-dimensional
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salivary cell clusters but also increased attachment and number of cell clusters. In summary, we
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demonstrated that fibrin hydrogel decorated with Laminin-111 peptides supports attachment and
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differentiation of salivary gland cell clusters with mature lumens.
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KEYWORDS: Salivary Gland, Laminin-111 Peptides, Fibrin Hydrogel, Rheology
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INTRODUCTION
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Proper salivary gland function is critical for oral health. Autoimmune disorders (such as
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Sjögren’s syndrome), genetic diseases (such as ectodermal dysplasia), and γ-irradiation therapies
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(for head and neck cancers) cause salivary secretory dysfunction and lead to severe dryness of
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the oral cavity.1-3 Dry mouth can lead to oral infections, sleep disturbances, oral pain and
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difficulty in chewing or swallowing food. 4-6 However, the current treatments for dry mouth only
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provide temporary relief and no tissue engineering approaches are currently available for patients
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suffering with dry mouth.7 Therefore, it is important to design a clinically safe matrix capable of
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supporting the growth of a functional salivary gland structure first in vitro and then in vivo
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applications.
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Previous studies showed that rat parotid gland (Par-C10) cells and mouse parotid cells form
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three-dimensional (3D) cell clusters displaying tight junctions (TJ) and agonist-induced secretory
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responses when grown on Growth Factor-Reduced Matrigel (GFR-MG).8, 9 Matrigel is rich in
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extracellular matrix (ECM) proteins, with the major components being Laminin-111 (L1) (60%)
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and collagen IV (30%). Although Matrigel allows the formation of 3D salivary constructs from
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single acinar cells, clinical application may be hindered by reports of basement membrane
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matrices supporting tumor growth. Also, it is derived from mouse cancer cells, which could
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trigger possible immune reactions in humans.10, 11
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Hydrogels are widely used as a tissue engineering scaffold.12 Among the hydrogels, fibrin
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hydrogel (FH) is the most extensively studied hydrogel. FHs are water-swollen, polymeric
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structures that form scaffolds capable of supporting cell viability and differentiation for long
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periods of time by interaction of cells with fibrin. Fibrin forms a hydrogel at physiological
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temperatures and contains native arginine-glycine-aspartic acid (RGD) sites that promote cell
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attachment.13 In addition, several studies demonstrated engineering of FH with conjugated
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growth factors, genes and recombinant viruses for multiple applications ranging from wound
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healing, vascular tissue engineering and lentiviral arrays. These include delivery of keratinocyte
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growth factor (KGF) to promote wound healing14, a peptide-TGF-β1 fusion protein to improve
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the contractile function, extracellular matrix synthesis and mechanical properties of vascular
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grafts15,
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microarray platforms 17-19.
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, and plasmid DNA and recombinant lentivirus for engineering gene delivery
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Previous studies also showed that a combination of GFR-MG and FH allowed Par-C10 cells to
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form 3D structures with a hollow lumen resembling salivary glands. Additionally, critical
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components within GFR-MG (i.e., a combination of EGF and IGF-1) enhanced salivary gland
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differentiation when polymerized within FH.8 However, EGF and IGF-1 were found to be
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incapable of independently producing organized cell clusters.8 More recently, another critical
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component of GFR-MG, L1 was able to produce organized salivary cell clusters using primary
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mouse submandibular (mSMG) cells.20 Nonetheless, the full L1 sequence may not be suitable for
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clinical applications, as some protein domains are known to promote tumorigenesis or
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immunogenic response that may outweigh the potential benefits provided by the whole
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molecule.21, 22 Conversely, the use of synthetic peptides is relatively simple and inexpensive as
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compared to animal derived proteins. In addition, controlled densities of peptides can be
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conjugated to the target material surfaces. Moreover, it is possible to minimize the immune
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reactivity or pathogen transfer.23 In 1999, Yoshida et al. reported that the YIGSR peptide has an
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inhibitory effect on tumor growth and an anti-proliferative effect.24 Moreover, the cell
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attachment and proliferation of mouse fibroblasts were improved on RGD-modified films in
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2012.25 Therefore, the use of a combination of peptides (RGD and YIGSR) within the L1
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sequence may provide the synergistic effects while minimizing the risks: a) the A99 (RGD)
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peptide corresponding to the α1 chain from L1 (important for cell adhesion),
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YIGSR peptide corresponding to the β1 chain from L1 (also important for cell adhesion,
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inhibitory effect on tumor growth and migration). 24, 26, 28
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and b) the
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The goal of this study was to test whether L1 peptides (corresponding to regions that promote
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intact salivary gland formation, see Table 1) were able to induce lumen formation in Par-C10
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salivary cell clusters. Our results indicate that cell clusters were formed on the FH modified with
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YIGSR peptide. Specifically, it improved morphology and lumen formation in rat parotid Par-
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C10 cells as compared to cells grown on unmodified FH. Moreover, a combination of YIGSR
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and A99 peptides not only allowed the formation of functional 3D salivary cell clusters, but also
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increased attachment and cell cluster numbers. In summary, FH decorated with Laminin-111
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peptides supports attachment and differentiation of salivary gland cell clusters with mature
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lumens.
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MATERIALS AND METHODS
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Materials
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Lyophilized fibrinogen from human plasma was purchased from EMD Millipore (Billerica,
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MA). Spectra/Por® 7 dialysis membrane (MWCO = 3.5 kDa) was purchased from Spectrum
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Laboratories (Rancho Dominguez, CA). Whatman™ syringe filter (0.8 µm) was purchased from
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GE Healthcare Life Sciences (Pittsburgh, PA). Millex syringe filter (0.22 µm) was purchased
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from Merck Millipore (Billerica, MA, USA). Paraformaldehyde (PFA) was purchased from
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Baker (Phillipsburg, NJ). Insulin-transferrin-sodium selenite media supplement, retinoic acid,
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hydrocortisone, gentamicin, epidermal growth factor (EGF) from murine submaxillary gland,
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DL-dithiothreitol (DTT) and ε-aminocaproic acid (εACA) were purchased from Sigma-Aldrich
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(St. Louis, MO). Rabbit anti-zonula occludens-1 (ZO-1) antibody was purchased from Invitrogen
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(Carlsband, CA). Dulbecco's modified eagle medium/nutrient mixture F-12 (1:1) (DMEM/F12
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(1:1)), fetal bovine serum (FBS), glutamine, Lab-Tek® chambered coverglass (8-well),
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sulfosuccinimidyl
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Fluor® 488 conjugated goat anti-rabbit secondary antibody, Alexa Fluor® 568 conjugated
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phalloidin, TO-PRO®-3 iodide nuclear stain and Fura-2-acetoxymethylester were purchased from
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Thermo Fisher Scientific (Newington, NH). Peptides were synthesized by University of Utah
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DNA/Peptide synthesis core facility.
6-(3'-(2-pyridyldithio)propionamido)hexanoate
(Sulfo-LC-SPDP),
Alexa
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Peptide Synthesis
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Two biologically active peptides derived from L1 were synthesized on an ABI431 or ABI433
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peptide synthesizer using a standard Fmoc solid-phase peptide synthesis as follows: Amino acids
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were protected at their amino terminus by the Fmoc (9-fluorenylmethoxycarbonyl) group and
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coupled to the growing chain after activation of the carboxylic acid terminus. Then, the Fmoc
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group was removed by piperidine treatment and the process repeated. After the peptide was
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assembled it was removed from the resin by treatment with trifluoroacetic acid (TFA). At the
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same time, protecting groups on amino acid side chains were removed yielding the crude linear
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peptide. Finally, one-step purification by reverse-phase HPLC yielded peptides with >95%
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purity. Two scrambled peptides were synthesized as a control. The overall synthesis scheme of
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scrambled peptides was the same as described above. All peptides were synthesized with a
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cysteine and two glycine residues (Cys-Gly-Gly, CGG) at the N-terminus. A cysteine free thiol
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group was used for coupling with thiol-reactive fibrinogen and the two glycine residues used as a
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spacer, respectively. A list of these peptides is shown in Table 1. Peptide
Sequence
Molecular mass
CGGALRGDN-amide
860.9
A99
L1 sequence Laminin α1 chain
(RGD)
(1145-1150) Laminin β1 chain
YIGSR
CGGADPGYIGSRGAA-amide
1350.5 (925-936) Scrambled peptide
RAD
CGGALRADN-amide
875.0 for A99 Scrambled peptide
SGIYR
CGGADPGSGIYRGAA-amide
1350.5 for YIGSR
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Table 1. Sequence of synthetic peptides
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Peptide Conjugated Fibrinogen
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Lyophilized fibrinogen was dissolved in 0.1 M Phosphate-Buffered Saline (PBS, pH 7.2, 0.15
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M NaCl, 1 mM EDTA) and dialyzed using a disposable cellulose membrane (MWCO = 3.5 kDa)
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overnight. Then, the fibrinogen solution was purified using a 0.8 µm filter. In order to produce a
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thiol-reactive fibrinogen, 7.2 equivalents of Sulfo-LC-SPDP was added to the purified fibrinogen
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solution and incubated for 1 h at room temperature. Subsequently, the excess Sulfo-LC-SPDP
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and its hydrolysis products (N-hydroxysulfosuccinimide, Sulfo-NHS) were removed by dialysis.
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The level of LC-SPDP-modification was determined by measuring the absorbance of pyridine-
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2-thione at 343 nm. Briefly, 10 µL of DTT (15 mg/mL) was added to 1 mL of modified
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fibrinogen. After 15 min of incubation, absorbance at 343 nm was measured and calculated the
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change in absorbance: ∆A343 = (A343 after DTT) – (A343 before DTT). The level of SPDP
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modification was calculated using the following equation: ����� �� � �� ���� �� � � ����� =
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∆���� 341 � � × (1) 8080 ��/�� �� � � �����
Where 341 kDa reflects the molecular weight of fibrinogen and the value 8080 reflects the extinction coefficient for pyridine-2-thione at 343 nm: 8.08 x 103 M-1 cm-1.29, 30
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For peptide conjugation, LC-SPDP activated fibrinogen was dissolved in 50 mM PBS (pH 7.2,
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0.15 M NaCl, 10 mM EDTA). Two equivalents of peptide per 2-pyridyldithiol groups of LC-
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SPDP-fibrinogen were added to the solution, and the mixture was reacted for 18 h at room
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temperature. The reaction was monitored by Tin-Layer Chromatography (TLC). Finally, the
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product was dialyzed against ultrapure water using a dialysis membrane (MWCO = 3.5 kDa) as
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described above and products were filtered using a 0.22 µm syringe filter from Merck Millipore.
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Then, peptide conjugated fibrinogen was lyophilized and stored at - 80 ºC until use.
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The concentration of fibrinogen was calculated using the following equation:
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" � ����� (��/��) = 1 2
Where ℇ*+,
,
the
extinction
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�#$% ×
�&' ��"�('� (2) ℇ*+,
coefficient
at
280
nm
for
human
fibrinogen,
is
1.51 �� ��01 (�01.31
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Molecular Weight Determination
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Static light scattering has been used to determine the size and molecular weight of
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macromolecules since the 20th century.32 When the light hits a macromolecule (e.g., a polymer or
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protein), some of the light is absorbed and re-emitted in all directions. The Rayleigh equation (3)
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describes the relationship between molecular weight and scattered light. By using this equation,
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the molecular weight of the modified fibrinogen can be determined. 2�3�� �ℎ 56&�' �� ∶
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Where:
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K is an optical constant
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C is the sample concentration,
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θ is the measurement angle,
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Rθ is the Rayleigh ratio,
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M is the molecular weight,
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A2 is the second virial coefficient.
89 1 = ; + 2�# 9> (3) 2:
