Assessment of hepatocellular function within PEG hydrogels
http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6TWB-4KXDWJ4-3&_coverDate=01%2F31%2F2007&_alid=508921244&_rdoc=1&_fmt=&_orig=search&_qd=1&_cdi=5558&_sort=d&view=c&_acct=C000059607&_version=1&_urlVersion=0&_userid=4420&md5=0a6bb7dc1ed695e1446012bbc052fe98
Tissue engineered liver has the potential to replace organ transplantation; however, due to the complexity of liver structure and function, fabricating the hepatic tissue is very challenging. This paper illustrate the utility of photopolymerizable poly (ethylene glycol) hydrogels for 3D encapsulation of heptic cells.
In this paper, they studied the survival and function of hepatic cells within the PEG hydrogel platform. They seeded bipotential mouse embryonic liver (BMEL) and Fibroblasts making Hepatocytes and Fibroblasts co-cultures (were seeded at a density of 5.0X105 cells/well, absorbed with 0.13mg/mL Collagen-1 extract from rat tail tendons) in PEG hydrogel platform, then, performed encapsulation of BMEL cells and primary hepatocytes. The cell viability was examined using calcein AM and ethidium homodimer fluorescent stains; also, performed RT-PCR to analysis gene expression and short interfering RNA transfection. To assess hepatocellular function and albumin release, used ELISA method, an enzyme linked immunosorbent assay. Found that the encapsulated BMEL aggregates and displayed a substantial induction of both albumin and alcohol dehydrogenase, which are both important markers of hepatocyte differentiation. So, this exhibited that BMEL cells can differentiate within PEG hydrogel plateform. Survival of PEG hydrogel encapsulated BMEL cells, for monodispersed cell culture, after one hour the viability was high of a 95%. However, after 3 days of post-encapsulation, the viability dropped down to 25%. As for pre-aggregated BMEL cells showed a significant increase in viability. This demonstrated the cell-cell interactions in maintenance of BMEL viability.
Also, to demonstrate the efficiency of siRNA-mediated gene knockdown for the hydrogel encapsulated BMEL cells, they examined slicing efficiency for a representative gene, lamin A. Found that the hydrogel encapsulation does not directly affect the maintenance of gene knockdown. This shows the compatibility of BMEL cell differentiation with hydrogel culture and the capacity to regulate gene expression through RNA interference.
I choose this paper because my final project is testing the hepatocyte’s ability to survive in agarose gel culture, which is similar with what this paper described. We tested the expression of albumin by RT-PCR, which is similar with what the paper did. Also, we measured the cell viability and the albumin production rate each time frame per cell. In our project, we used partially collagen I mixture with agarose to make the 3D culture. We observed that the culture with collagen I tend to have cells clumping together, and have better survival rate than the agarose only culture. This is also observed in this paper where they demonstrated the cell-cell interactions in maintenance of BMEL viability.
Saturday, December 16, 2006
Injectable Liver: A Novel Approach Using FibrinGel as a Matrix for Culture and IntrahepaticTransplantation of Hepatocytes
TISSUE ENGINEERINGVolume 11, Number 11/12, 2005
http://www.liebertonline.com/doi/pdf/10.1089/ten.2005.11.1718
In this paper, the researchers tried to focus on cell transplantation and tissue engineering techniques with liver cells as experimental therapies for some liver diseases. They made fibrin-based gel matrix as carrier for hepatocytes in culture. Then they developed a direct injection technique to take hepatocytes harvested from rats. After cell isolation, they did PKH26 labeling. Adult Sprague-Dawley rats were used as organ donor and recipients. For cell transplantation, a minilaparotomy was performed; the cell-matrix mixture was injected directly to the organ. After different time harvest, animal were killed and liver were removed and to take histological investigation. DNA quantification was preformed and cell numbers showed the viability. In another hand, they did RNA extraction, cDNA synthesis and PCR (RT-PCR). The explanted liver tissue was snap frozen in liquid nitrogen. Cytospins, fixtion, histology, and immunohistochemistry were preformed on the tissue. In the end, statistical analysis provide the results.
From the experiments they did above, they drew some results. Cell numbers were assessed by DNA content, they showed the viability of the cells is good, which means fibrin matrix is an appropriate environment for hepatocytes. Fluorescence microscopy of the liver was performed to identified PKH26 labeled cells. RT-PCR and IH showed preservation of hepatocytes and hepatic stellate cells into the host liver. Direct injection technique of the fibrin gel-immobilized hepatocytes is technically feasible. They concluded that fibrin gel immobilization is an good tool for develop tissue engineering artificial liver system. They also discussed the fibrin glue as a matrix supportive of hepatocytic differentiation, using fibrin glue as a carrier for injectable liver, and remolding of liver tissue after injection of fibrin-hepatocyte mixture.
I chose this paper, since it’s really similar to what we are doing in the final project. These German researchers used fibrin gel as matrix, we did use agarose gel to culture cells. They did future steps to seed the culture into rats and gave a normal better modeling environment, which is more worth us to think about. We are performing most of their cell analysis techniques, which we can watch as references such as RT-PCR, Cell counting and immunohistochemistry. We can do a lot of comparison and contracts between our projects and theirs. Their results are good, which mean other gel than collagen can work with liver cells. This gives us motivation to see our result on agarose gel. In the end, their discussions are also very advisable.
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Sunday, December 03, 2006
Development of a Closed Bioreactor System for Culture of Tissue-Engineered Skin at an Air–Liquid Interface
(This is Terry posting on the behalf of Elena, who's having blogger problems.)
Before autologous tissue-engineered skin providing a reasonable barrier can progress to the clinic, it is needed to design bioreactor that can construct cells at an air-liquid interface. This article investigates and compares the designs for continuous as well as batch-reaction bioreactors. A comparison between continuous perfusion with medium versus changing medium every few days was also used to determine which method would better support metabolic activity.
Four different scaffolds were used in this study: acellular deepidermized human dermis (DED), electrospun polystyrene (PS; 0.8–1.0 mm thick), a composite of electrospun poly-DL-lactide fiber and polystyrene (PDLA/PS) (0.8–1.0 mm thick), and a commercially available nonwoven scaffold (Azowipes). Normal human keratinocytes and fibroblasts were isolated and cultured and the viable cell density was assessed by MTT-ESTA (an assay based on the conversion of MTT to a colored formazan end product by intracellular dehydrogenase activity). Viability measurements by MTT indicated that fibroblast and endothelial single cultures preferred submerged culture conditions, whereas an air–liquid interface gave greater total cell viability for the single culture of keratinocytes and fibroblast–keratinocyte cocultures compared with submerged cultures. MTT measurements showed that total cell viability of fibroblast–keratinocyte cocultures was significantly higher in PS and PDLA/PS compared with DED.
Results also indicated that the cell viability of tissues cultured under continuous perfusion was significantly higher than that of tissues cultured under batch-fed culture (Fig. 5). It was noticeable that total cell viability was almost 2-fold higher for PS electrospun scaffolds with continuous feed versus DED with continuous feed. In the case of keratinocytes this may result in cells failing to proliferate or it may induce premature abnormal differentiation. Thus, continuously perfused medium is likely to be more effective than frequent changes of static culture medium every few days.
Overall, the bioreactor developed in this investigation shows several technical and operational advantages that will be of significance for skin tissue-engineering research. These advantages include: a completely closed system, a bioreactor that can be operated easily under sterile conditions, a design the potential for parallel connection of individual chambers, allowing for multiple experimental reactors to be stacked vertically and therefore minimizing culture space, and a bioreactor with multiple chambers to allow for simultaneous experiments.
I chose this article due to its relevance to cell-culture techniques used during our lab. The feeding technique use din lab consists of changing the medium every few days, however in this report, it is suggested that a continuous perfusion of medium resulted in an increased cell viability. In addition, this investigation focuses on an air-liquid interface cell culture, which would be needed in tissue-engineered skin to be produced for clinical use. This aspect relates to our project of tissue engineering dermis and can provide insight as to possible future work that could provide better results.
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Monday, November 13, 2006
Reduced contraction of skin equivalent engineered using cell sheets cultured in 3D matrices
http://www.sciencedirect.com/ (search for title above)
or
The cell sheets that have been tissue-engineered in the past few years have had poor mechanical properties. Because of the fragility of cell sheets, external supports such as stainless steel rings and non-degradable polymeric membranes have to be used. In this experiment, they used two different types of 3D matrices with cultured fibroblast sheets to form a possible tissue engineered skin replacement that have the mechanical properties more similar to native skin. These would maintain their regenerative capacity while also showing reduced wound contraction when transplanted in vivo. The two 3D matrices they used were a weft-knitted poly (lacted-co-glycolic acid) mesh (PLGA), which has mechanical properties similar to native skin while also supporting dermal fibroblast attachment and proliferation, and a collagen sponge crosslinked with hyaluronic acid (CHA), which has greater resistance to enzymatic degredation along with reduced swelling.
The drawback in using cell sheets is that the poor mechanical properties results in difficulty in handling the sheets along with extensive contraction . The results of the expirement showed that the weft-knitted PLGA mesh was better than the CHA sponge because it provided high flexibility that was mechanically stable as a graft. The PLGA-cell sheet showed contraction comparable to autografts. These PLGA-cell sheets contracted less compared to using PLGA alone, showing a synergistic effect between the PLGA mesh and the cell sheets in preventing contraction in a wound, which would lead to less scar formation. The CHA matrix didn’t show great results in vivo because of its rigidity, which prevented it from adapting to the movement of the animals that resulted in wound healing under the matrices instead of over the matricies.
I chose this paper because our project is on TE skin. Although we won’t have a chance to experiment much using different types of 3D matrices like in this experiment, I thought it was a good reminder for us to think of design principles for our devices that can be used clinically in the real world. Even if we were to eventually create a skin sheet that showed nearly all the biological and chemical properties of natural skin tissue, putting the device into a patient for them to actually use is another huge consideration. If the device can’t be placed in a practical and viable way, then it is pretty much useless. It was also interesting to see the thought process of the entire experiment because they used a wide range of laboratory techniques, most of which we learned throughout the semester (cell culture, mechanical properties, microscopy, antibodies, etc.).
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Cell-cell Interactions Are Essential for Maintenance of Hepatocyte Function in Collagen Gel But Not on Matrigel
Prabhas V. Moghe, Robin N. Coger, Mehmet Toner, Martin L. Yarmush
Full text at: http://www3.interscience.wiley.com/cgi-bin/fulltext/71004078/PDFSTART?CRETRY=1&SRETRY=0
Given the potential pharmacological, toxicological, and therapeutic potential, hepatocytes are often cultured on collagen as a monolayer and or induced three-dimensional aggregates. The study compared the importance of cellular aggregation and seeding density in two different hepatocyte culture systems, the two-dimensional monolayer in a collagen sandwiches and three-dimensional aggregates induced by the mouse sarcoma derived Matrigels. In order to determine the effectiveness of each of these systems in retaining hepatocyte function, the culture medium was measured for rat serum albumin content by enzyme-linked immunosorbant assay (ELISA) with purified rat albumin and peroxide-conjugated antibody and DNA content analysis.
Upon culturing, the hepatocytes cultured in the collagen sandwich after 10 days appeared more flattened and exhibited bright cell-cell contacts compared to the hepatocytes cultured in the Matrigel, where they appeared round and formed comparatively large three-dimensional aggregates. Albumin secretion were obtained each day for five different seeding densities (1.75, 3.5, 7.0, 17.5, and 70.0 x103 cells/cm2) and normalized to the amount of DNA present within each culture as obtained by the DNA content analysis. With high cell seeding densities the, both cultures exhibit similar levels in elevated function. However, as the cell seeding densities decreases, the collagen sandwich cultures exhibited a rapid deterioration in albumin secretion while the Matrigel cultures maintained similar levels of albumin secretion.
The decreasing secretion levels in the collagen sandwich and the maintenance of secretion levels in the Matrigel may be associated with the differences between the cell-cell and cell-matrix contact levels in the two cultures. As a result of the different morphologies that the collagen sandwich and the Matrigel induce, cell-cell contact and cell-matrix contact varies differently between the two systems. In both systems, the cell-cell interaction parameter decreases with cell decreasing cell density. The cell-matrix interaction parameter, however, remain relatively unchanged in the collagen sandwich as cell density decreases whereas the cell-matrix interaction parameter increases in the Matrigel as the cell density decreases. Thus, the paper concludes that in collagen sandwich systems, the maintenance of hepatocyte function corresponds to the amount of cell-cell contact whereas hepatocyte function is maintained from matrix derived cues.
I chose this paper as, in the liver project, we are also testing the maintenance of hepatocyte function in a new matrix, agerose. However, we will be measuring albumin secretion rates using western blots and determining the number of viable cells after one week of culture using hemocytometer counts. This paper might provide insight into how cellular aggregation, seeding density, and the resulting cell morphology might affect rates of albumin secretion and hepatocyte functional maintenance in different culturing systems.
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The application of new biosynthetic artificial skin for long-term temporary wound coverage
Full text article:
visit: http;//www.sciencediret.com
and type in the above article
Skin acts as a barrier to keep antigens out of the immune system, and to keep bodily fluids in. Open wounds where the epidermal and dermal layers are absent are prone to infection and need to have the skin repaired immediately to restore homeostasis. The most ideal way to do this is for an autologous skin graft because immune rejection would not be a factor. However this is not always ideal if the wound is large. The authors of the paper investigate a new method of healing skin wounds with engineered artificial skin that will either 1) cover the wound long enough for the wound to heal naturally or 2) cover the wound long enough until an autologous skin culture can be grown to an amount that will suffice in a permanent skin graft.
The artificial skin consists of a thin layer of silicone fused with acellular porcine dermis (APD), and therefore sufficiently named silicone acellular porcine dermis (SAPD).
A 4cm x 5cm skin wound was delivered onto each back of 36 rats; half of them received SAPD treatment over the entire wound and the other half received Biobrane (a manufactured biosynthetic skin substitute that also contains silicone fused to dermal porcine substance).
The wounds were analyzed weekly over a 6-week period using pathological tests. The Biobrane group exhibited wound contraction and digestion of the dermal layer after the 3rd week of grafting. Before the dermal layer was digested, its porcine dermis component faced immunorejection and caused wound inflammation. On the contrary the SAPD group exhibited no wound contraction and after the 6th week, SAPD maintained its well-organized porcine dermis, thereby creating a dermal template that allowed the containing procine collagen to incorporate into the recipient’s wound. No immunorejection was present with minimal inflammation.
Although SAPD proves to be the better artificial skin graft in the observations, one of the major drawbacks is its time dependency. After the 6th week of grafting, the silicone layer separates from the APD, causing dermal layer exposure and infection. As long as the wound can heal or a skin culture can be grown within 6 weeks, SAPD is a sufficient skin graft.
This article was my pick of the liter because its subject matter was somewhat relevant to my project of tissue-engineered skin. The paper provided little insight on methods since our materials vary from those found in the paper, but it was helpful to learn that the dermal layer was the important factor in a successful skin graft – the epidermal layer (in this case silicone) was to provide protection and was not crucial in the material-recipient incorporation. Also it was interesting to know that there is still much headway that can be made with artificial skin despite it being the first tissue organ ever to be engineered.
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Sunday, November 12, 2006
Physiologicallly relevant increase in temperature causes an increase in intestinal epithelial tight junction permeability
Karol Dokladny, Pope L. Moseley and Thomas Y. Ma
Am J Physiol Gastrointest Liver Physiol 290: 204-212,2006
http://ajpgi.physiology.org/cgi/content/full/290/2/G204
This paper discusses the impact of physiologically relevant increase in temperature (37 -41 degrees in Celsius) on epithelial tight junctions as well as the role of heat-shock proteins (HSPs) in regulating this heat stress. The study was done using a cell line known as caco-2 cells. Non-leaky epithelial tight junction barrier is "crucial in providing barrier function against epithelial penetration of pathogenic bacteria and toxic luminal antigens like endotoxins." As indicated by the study, the disruption of the tight junction barrier results in a "leaky" barrier that allows paracellular permeation of toxic luminal substances. The experimental data presented in the paper show that HSPs play an important protective role in preventing heat-induced disruption of the tight junction.
Western blot analysis was used to assess the HSP, occludin, ZO-1, and beta-actin protein that were expressed just as we did in lab. The researchers mixed the clear lysate derived from a centrifuged cell lysate with a Laemmli gel buffer, boiled for 7 minutes, and lated separated using SDS-PAGE gel. The protein from the gel was transfered to Nitrocellulose membrane overnight.
This paper was very interesting to me because it serves as a cautions to me as prospective tissue engineer to be mindful of little things that might end up ruining my engineered tissue. I was also intrigued by its mention as well as usage of certain techniques that I have learnt in class.
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Friday, November 10, 2006
Autologous cartilage implantation (ACI) is a new medical alternative that especially benefits for patients who have a damaged cartilage. The goal of ACI is to provide the patient with a durable, load bearing functional joint surface by the repair of articular carticular with both biomechanical and histologic characteristics comparable to normal articular cartilage. There are two stages involved in this ACI procedure. First, some health cartilage cells are collected from the patient’s knee. Then, these biopsytissue are sent to a special laboratory to grow for weeks and transplant back to the patient’s damaged region for new cartilage regeneration. One of the advantages of ACI is the usage of the patient’s own cells could reduce the chances of infection. Besides, ACI has the ability to restore hyaline-like articular cartilage.
ACI is an advanced, cell-based orthobiological technology; however the quality of this treatment is still not very well determined. In this article, “Autologous Chondrocyte Implantation: Superior Biologic Properties of Hyaline Cartilage Repairs,” by Henderson I, Lavigne P, Valenzuela H, and Oakes B. (could be downloaded from https://webfiles.berkeley.edu/wincheung/shared/ ), the properties and qualities of ACI were tested and analyzed. The authors focused on three points. First, the different effects resulted from cartilage repairs of different tissue types in terms of stiffness and outcome. Second, the correlation between the anatomic locations and the properties of the repairs. Third, the correlation between the presence of an abnormal macroscopic appearance at arthroscopy and its biomechanical or histologic properties. The results were based on two standard scoring systems. The International Cartilage Repair Society (ICRS) visual scoring system and the International Knee Documentation Committee (IKDC) score, which evaluate the symptoms, activity level, and health-related quality of life measures.
There were two limitations in this study. First, among the symptomatic population, which the data were derived from, they had additional abnormalities unrelated to the ACI repair. This made the results obtained from them couldn’t easily be extrapolated to the asymptomatic population with ACI. Second, the limitation to study the potential relation between the repair’s biologic properties and the clinical outcome due to the indentometry had to base on proper instrument positioning and also the repair thickness, which could possibly cause inaccurate measurements. Although the histologic evaluation was based on a 2mm thick tissue sample, this couldn’t represent the total composition of the repair tissue, it is more adequate to test for reliable, reproducible, and repeatable results.
It was found at the average of 26.5 months after implantation, the repair was stiffer than normal cartilage. The greatest stiffness was recorded in the following orders: the hyaline articular cartilage, hyaline-like, fibrocartilage, hyaline-like/fibrocartilage group. Besides, there were no difference in the histologic quality resulted from the difference anatomic location of the repair. Regarding of the third focus of the study, the relationship between the presence of an abnormal macroscopic appearance at arthroscopy and its biomechanical or histologic properties, the ICRS and IKDC scores were inconsistent. Based on the ICRS scores, the patients who were macroscopically normal had greater maximum and normalized stiffness than patients who were macroscopically abnormal. On the other hand, the patients with or without abnormal macroscopic appearance scored no difference in IKDC scores. The IKDC scores increased with time in patients in both cases, hyaline cartilage and fibrocartilage. These scores indicated patients did well regardless of the quality of the repair at 3 years postoperatively because these scores were comparable to scores of asymptomatic patients in the ACI cohort. 24 months after ACI, the overall stiffness and macroscopic appearance of hyaline articular cartilage and hyaline-like repairs were similar to normal articular cartilage.
My grandma has inspired me to have a special interest in the field of tissue engineering, and be more specific – cartilage, because of her knee pain. Her cartilage is wearing out as a result of aging, and by the time I heard this ACI repair treatment, I thought it might bring hope to save my grandma from pain. Treating ACI as a possible treatment for my grandma, I want to know more about ACI, and that’s why this article was especially attractive to me because it fulfilled my curiosity about the quality of ACI repair. Besides, by knowing these mechanical and histologic properties of current ACI, we can make improvement and hence one step closer to the durable cartilage repair.
Yee-Wan (Win) Cheung
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Viscoelastic Testing Methodologies for Tissue Engineered Blood Vessels
Joseph Berglund, Robert Nerem and Athanassios Sambanis
Journal of Biomech Engineering 2005 Vol 27
http://scitation.aip.org/getabs/servlet/GetabsServlet?prog=normal&id=JBENDY000127000007001176000001&idtype=cvips&gifs=yes
Matching the complex mechanical behavior of native blood vessels is one of several obstacles in creating a suitable tissue engineered blood vessel. Many of the TE vessel mechanical testing methodologies have used single-point burst pressures measurements and uniaxial tensile testing as an indication of mechanical suitability. However,since blood flow is a pulsatile behavior, and native blood vessels exhibit a time-varying behavior, other methods are needed to correctly characterize the mechanical properties of TE vessels. In addition to performing uniaxial tensile testing, this paper reports the use of viscoelastic characterization methods to model the time-dependent behavior of TE and native vessels.
TE vessels were made from rat collagen (2 mg/ml) and human dermal fibroblast (1 x 106 cells/ml). TE vessels were made to form a tubular structure with a 3mm inside diameter. Some TE vessels were combined with acellular support sleeves made from untreated and glutaraldehyde crosslinked collagen. Common carotid arteries were taken from 1 to 2 year old pigs.
Uniaxial tensile testing was used to measure overall strength (ultimate tensile strength). Stepwise stress relaxation and creep testing was performed (for more details see paper link). Mathematical modeling, using 3 and 4 parameter constitutive, models was used to characterize stress relaxation and creep data.
This paper also reports geometrical changes for all samples after 8 and 23 days in culture. Interestingly, this study found that the addition of acellular support sleeves had minimal effect on gel compaction. However, a difference in mechanical properties was observed amoung the samples. The Glutaraldehyde treated vessel constructs exhibited the highest burst strength but were still inferior to the native arteries. The untreated vessel constructs seemed to match the overall behavior of the native vessels the best.
I chose this article because it provides a framework for characterizing the mechanical suitability of TE vessels. It also illustrates the use of mathematical models which is something of interest to me.
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Monday, November 06, 2006
Toshihiro Izumi, Toshiyuki Tominaga, Junichi Shida1, Futoshi Onishi & Moritoshi Itoman Department of Orthopaedic Surgery, Kitasato University School of Medicine,
1-15-1 Kitasato, Sagamihara, Kanagawa 228-8555, Japan
http://www.springerlink.com/content/g523121861680452/fulltext.pdf
Cartilage graft is a common technique applied in repairing chondral or osteochondral defects. One way of performing cartilage graft is by autologous chondrocytes transplantation following cell culture. However, one of the potential problems of this method is that chondrocytes may change their phenotype during monolayer culture. To solve this problem, the experiment presented in this research paper hypothesized that chondrocytes cultured over agarose (suspension culture) as a source of graft material can retain the expression of type II collagen and glycosaminoglycans, and the expression of these two products for chondrocytes cultured in a plastic glass (2D culture) is also measured as a control.
105 cells/cm2 of rat chondrocytes are isolated from coast cartilage and are dispersed in Ham’s F-12 medium supplemented with 0.2 mg/ml bovine serum albumin, 50 mg/ml ascorbic acid, antibiotics–antimycotic, 10% fetal bovine serum ,and 25mM HEPES, pH 7.4. The isolated cells were collected, and seeded on six well plate either uncoated or precoated with 1.5% agarose. Chondrocytes cultured in uncoated dishes represented the monolayer culture, while chondrocytes in coated dishes represented suspension culture. Cultures were then maintained in a humidified atmosphere consisting of 95% air and 5% CO2 at 37 oC. Cells were cultured for two weeks, and medium was changed twice a week. After 14 days in culture, the expression of glycosaminoglycans is examined by a histochemical test in which the chondrocytes are stained with safranin O (a biological stain used in histology). On the other hand, the expression of type II collagen is examined first by an acid guanidinehiocyanate–phenol–chloroform method for RNA extraction and following by northern analysis. The cultured chondrocytes are then transplanted to a rat with osteochondral defects.
The result of this study shows that chondrocyte phenotype was maintained in suspension culture over agarose, as assessed by northern analysis and histochemistry compared with chondrocyte monolayer culture. Moreover, this study shows that suspension culture chondrocyte grafts in femoral osteochondral defect also resulted in hyaline cartilage formation compared with controls in this study. Surface of the condylar defect was smooth, and the matrix produced in the defect contained glycosaminoglycans.
The reasons I choose this paper are because it is related to our project and may provide some clues to accomplish the objects in our experiment. Instead of concerning the mechanical properties of the chondrocytes / agrose cell culture, measuring the expression of collagen II of our chondrocytes after one week of culture is also the other big challenge in this project. This problem can get complicated as we do not know which portion of the collagen is from the calf serum and which portion is from the cells. Therefore, solely running the sample and a negative control in western blot cannot tell us whether the cells are expressing collagen II or not. The application of northern blot used in this paper suggests a possible way to deal with this problem since the mRNA of collagen II would only come from the chondrocytes. Nevertheless, we still have to come up with some ways to quantify the protein.
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Engineering Vascularized Skeletal Muscle Tissue
Nature Biotechnology 23, 879 - 884 (2005)
Shulamit Levenberg, Jeroen Rouwkema, Mara Macdonald, Evan S Garfein, Daniel S Kohane, Diane C Darland, Robert Marini, Clemens A van Blitterswijk, Richard C Mulligan, Patricia A D'Amore & Robert Langer
Full Text: http://www.nature.com/nbt/journal/v23/n7/full/nbt1109.html
Vascularization is a critical factor in the viability of bioenegineered tissue. In relatively thin tissues with low metabolic activity such as skin, little vascularization is required. Yet in thicker tissues that require a large supply of nutrients and removal of waste, vascularization has been a critical road block in achieving clinical viability.
In most tissue engineering transplantations, vascularization occurs post implant via the host and through the addition of growth factors. Unfortunately this technique has not been successful for large, thick tissues. The other option for tissuevascularization is to begin the process prior to implantation. In the paper, "Engineering vascularized skeletal muscle tissue," Levenberg etal. were able to produce prevascularization prior to implantation and viability post implantation in an in-vivo model.
The first step in the experiment by Leavenberg was creating a co-culture of muscle and endothelial cells. When co-cultured and analyzed over time endothelial tubes formed around the elongated muscle cells showing the beginings of vascularization. This concept was then extended by culturing three different cells together; skeletal muscles, endothelial cells, and fibroblasts. The fibroblasts were added due to their ability to differentiate into smooth muscle cells, which would act to stabilize the endothelial tubes. This tri-culture showed even greater stabilization then the co-culture with the presence of smooth muscle cells and also the increased production of angiogenic growth factors such as VEGF. Having shown proof of concept in-vitro the tri-cultured tissues were then implanted into mice.
In the mice three different sites received tissue, one of which was abdominal muscle. The implant showed evidence of viability, and very interestingly, it appeared that the new muscle appeared toalign with the fibers of the host tissue. This revealed the possibility of both functionality and viability in the implant.
The study by Levenberg etal. was one of the first to show the ability to create prevascularization in thick complex tissues. The results of this research creates great possibilities for advancement of tissue engineering in such complex metabolically active tissues as liver or brain. In addition, the techniques developed could be used for studyingmulticellular processes, such as angiogenesis in-vitro.
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Nano neuro knitting: Peptide nanofiber scaffold for brain repair and axon regeneration with functional return of vision
Kwok-Fai So, and Gerald E. Schneider
Rutledge G. Ellis-Behnke, Yu-Xiang Liang, Si-Wei You, David K. C. Tay, Shuguang Zhang,
doi:10.1073/pnas.0600559103
PNAS 2006;103;5054-5059; originally published online Mar 20, 2006;
http://www.pnas.org/cgi/content/full/103/13/5054
This paper discusses the regeneration of the optic nerve by aiding neuron reconnection on a nanometer scale scaffold created from amino acids. The experiment consisted of severing optic nerves in hamsters and then patching them with a self assembling peptide nanofiber scaffold (SAPNS). The reason for choosing such a scaffold is motivated by the inert properties of amino acids in the cellular environment. This scaffold also provides nutrients for growing cells and aids in the healing of the wound.
This article suggests also that nerves can be reattached using cell grafts from nerves in the legs of the animal. This is not as desirable as the SAPNS method as legs are often damaged by such a process. Tests were done after 30, 45 and 90 days and healing evidence was found. Imaging with an SEM and optical microscopes of the wound area also showed the SAPNS aiding in the healing of the nerve cells.
I chose this article because I think it is interesting. Scaffolds for engineered cells are almost as important as the growth of the cells. A biologically and chemically inert scaffold that functions on the nanometer scale is something that could benefit many tissue engineered devices at a variety of size scales.
I am skeptical about the results of the paper. The movies that show the hamster reactions are hard to quantify, and the possibility of another means of neuron regeneration was largely disregarded or not even mentioned to be as likely as the SAPNS aiding growth method. However, the paper does detail the experiment well and discusses the insertion of the scaffold into the wound and the various controls they used to eliminate random hamster visual artifacts. There is also visual evidence of the growth.
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Sunday, November 05, 2006
Compressive Strains at Physiological Frequencies Influence the Metabolism of Chondrocytes Seeded in Agarose
David A. Lee and Dan L. Bader
Full text link: http://www3.interscience.wiley.com/cgi-bin/fulltext/109929044/PDFSTART
The experiment presented in the article studies the universality of mechanotransduction pathways for chondrocyte metabolism under the application of static and dynamic mechanical strains. Specifically, the experiment aims to characterize whether chondrocyte deformation under mechanical strain has the capability of stimulating three major markers of chondrocyte metabolism: proteoglycan synthesis, cell division, and protein synthesis.
In the experiment, static and dynamic mechanical strains were applied on agarose-chondrocyte cylinders using a specially designed cell straining apparatus. The level of gross compressive strain used was 15%, which lies in the middle of the 0-30% physiological range for cell strain in intact cartilage subjected to physiological loads. For dynamic loading, the frequencies studied were 0.3 Hz, 1 Hz, and 3 Hz – all three were within the physiological range. The agarose-chondrocyte cylinders were prepared from chondrocytes removed from the metacarpophalangeal joints of 18-month-old steers, embedded in 3% agarose, and cultured under strain for 48 hours in DMEM with 20% fetal calf serum. Unstrained agarose-chondrocyte cylinders were used for control.
Chondrocyte viability was determined for each of the experimental group using trypan blue assay and the results showed that viability ranged from 97.8 to 99.1% of the time-zero viability. Glycosaminoglycan (GAG) synthesis by chondrocytes embedded in agarose was determined using a rapid spectrophotometric procedure that involved papain digestion of tissue or culture medium that provides glycosaminoglycans for assay. The results, normalized to the control cultures, indicated a significant reduction in glycosaminoglycan synthesis for static strain and 0.3 Hz dynamic strain, but a stimulation of glycosaminoglycan synthesis to 40% more than the unstrained control for dynamic strain at 1 Hz. Dynamic strain at 3 Hz did not significantly alter glycosaminoglycan synthesis. Incorporation of [3H]thymidine was analyzed as a marker for cell division and the results showed that its uptake was inhibited in cylinders subjected to static strain as compared to static strain, but was stimulated in cylinders subjected to dynamic strain at all three frequencies. Finally, incorporation of [3H]proline was analyzed as a marker for protein synthesis. The results showed that when compared to unstrained control, [3H]proline uptake was inhibited in cylinders subjected to both static and dynamic strain at all frequencies investigated. Because the three parameters investigated in the study were each influenced by the strain regimens in a distinct manner, it was concluded that that the mechanotransduction pathways involved were likely to be uncoupled.
I chose this article because I feel that this study is particularly important for the development and design of cell-seeded cartilage repair systems for cartilage diseases such as arthritis. As a matter of fact, a balance between cartilage matrix synthesis and degradation is critical both for the maintenance of articular cartilage function and skeletal development and growth. Because the focus of this study is on the mechanical aspects that can alter this balance, it is thus able to provide a general understanding of chondrocyte regulation in cartilage when subjected to various types of compressive strains. Additionally, the results from the study can give insights on how a tissue engineer can design an experiment that closely mimics human physiological conditions. The study presented made this attempt by subjecting the chondrocyte cell culture to dynamic loading at various frequencies so that it is more similar to normal walking. This way, more applicable results can be drawn from the experiment that can be used to generalize the effects of mechanotransduction on articular cartilage under physiological loading in human joints.
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Saturday, November 04, 2006
Reduced Contraction of Skin Equivalent Engineered using Cell Sheets Cultured in 3D Matrices
Full Text available at following link:
http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6TWB-4K18VTF-2&_coverDate=09%2F30%2F2006&_alid=481170456&_rdoc=1&_fmt=&_orig=search&_qd=1&_cdi=5558&_sort=d&view=c&_acct=C000059607&_version=1&_urlVersion=0&_userid=4420&md5=36f4a4e1bea9fa127e704ef716f0eb78
The main objective of the experiment described by this paper was to improve the mechanical properties of cell sheets used to generate tissue engineered dermal equivalents. Cell sheets have been used for a variety of tissue engineering purposes that range from artificial blood vessels to myocardial patches and artificial skin. While they have the advantage that the cells on the sheet can be used to engineer a natural neo-tissue, a major shortcoming of cell sheets is that they contract when removed from culture surfaces, causing graft sizes to be reduced. Cell sheets are also very fragile and difficult to handle. This paper describes a technique for resolving these shortcomings in which human fibroblasts sheets are cultured in combination with three-dimensional matrices to form a contiguous dermal construct that does not contract over time.
The group in this study hypothesized that fibroblast sheets grown in conjunction with three-dimensional matrices will maintain their regenerative capacity and result in reduced wound contraction. To test their hypothesis they used their technique with two kinds of 3D matrices: a PLGA scaffold, and a collagen sponge cross linked with hyaluronic acid (CHA). I won’t go into to much of the details of their materials and methods, but I will note that the 3D matrices and cell sheets were fabricated separately, at which point cell sheets were peeled off the Petri dishes on which they were grown and then folded over the matrices to from the 3D dermal equivalent. Human keratinocytes were then seeded on top of each dermal equivalent and allowed to culture for seven days. The constructs were then either raised in an air-water interface for four weeks to induce cell stratification, or they were transplanted onto full-thickness wounds in nude rats for four weeks.
In the end, both PLGA and HCA constructs to varying degrees came to resemble human skin with mechanical properties far more stable than those inherent to cell sheets alone. Each possessed a stratified keratinocyte layer that resembled native epidermis. In addition, cell migration of the fibroblasts from the sheet into the 3D scaffold was observed for both PLGA and HCA, creating a 3D matrix of fibroblasts resembling that of the dermis. However, following transplantation, it was found that the CHA sponges sloughed off the wound within two weeks. The PLGA scaffolds, in contrast, took after 1 week post-transplantation and registered a take rate of 100%. Wounds re-epithelialized 3 weeks after transplantation. This demonstrates both the successes and failures of the experiment. While both constructs exhibited properties that mimicked those of human skin, in the end it was found that the CHA matrix did not take due to its higher than normal rigidity, which prevented it from conforming to changing wound topography as the animals moved.
I chose to post this paper because of the similarity of its objectives with those of our class project as applied to tissue engineered skin, in addition to the fact that many of the methods that were used to characterize their 3D constructs were similar to or the same as the techniques that we have learned in this course. Like our project, the objective of the experiment described by this paper was to create a 3-dimmensional skin substitute that is easy to work with and has mechanical properties comparable to those of the dermis. To accomplish this, they had to characterize their construct by observing the cells using microscopy and ensure that the fibroblasts were correctly distributed in their 3D matrix. In addition, like we have done in class, they used immunostaining techniques to verify that their cells were continuing to express their proteins of interest and generating a matrix that resembled that of human skin.
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Thursday, November 02, 2006
Human Tissue Engineered Blood Vessel For Adult Arterial Revascularization
Full text available at:
I chose this article for two main reasons. First of all, I believe that it would be helpful to other Bioengineering 115 students whose projects focus on tissue-engineered blood vessels. Besides that I think this article is a very comprehensive one. It thoroughly describes the technique for preparing and testing one particular type of the TEBV (tissue-engineered blood vessel).
In the experiment described human skin fibroblast cells were isolated from bypass patients and then cultured into sheets. Complex media supplemented with bovine serum, glutamine, penicillin, streptomycin and sodium ascorbate was used to feed the culture. As in natural blood vessels, three distinct cell layers (living adventitia, decellularized internal membrane and endothelium) were formed in the TEBV. Temporary Teflon®-coated stainless steel tube was used as a mechanical support during the formation of the first two layers (adventitia and IM (internal membrane)) and was removed later. When the vessel was ready, the natural conditions were simulated by subjecting the TEBV to the pulsating stream with the flow rate varying from 3ml/min to 150ml/min.
Mechanical testing was conducted to estimate (1) the burst pressure and (2) the suture retention strength of the vessels. Compliance was calculated based on the change in vessel diameter in response to increasing pressure (high resolution digital imaging was used to measure the vessel diameter).
The final phase of the experiment involved canine, nude rats and primate studies. In all trials immunosuppressive drugs were administered prior and following the introduction of the TEBV into the body. Tissue fixation and histology at different time periods were used to examine the condition of the newly incorporated blood vessels. The analysis revealed successful tissue integration, vasa vasorum formation and cell accumulation on the luminal side of the IM. Furthermore, the shape and size of the TEBV was approximately unchanged and proteoglycan expression was suppressed. This is indicative of the relative success of the preclinical trials.
In the end, authors suggest that if clinical trials of the TEBV prove successful further research should focus on decreasing time for the vessel production and other applications of allogeneic TEBVs.
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Biochemical and Functional Changes of Rat Liver Spheroids During Spheroid Formation and Maintenance in Culture: I. Morphological Maturation and Kinetic Changes of Energy Metabolism, Albumin Synthesis, and Activities of Some Enzymes
Mingwen Ma, Jinsheng Xu, and Wendy M. Purcell
http://www3.interscience.wiley.com/cgi-bin/abstract/106563224/ABSTRACT?CRETRY=1&SRETRY=0
There have been many studies in the past observing how liver cells function when cultured on monolayers. Cells that aggregate into spheroids function much longer and superior (liver-like) to those cultured as monolayers in a dish. Spheroids are gobular formation of cells that form a three-dimensional, multicellular aggregate. Such a formation is favored for the cells will maintain cell-cell contact and maintain more liver-specific functions, as in secretions. Nevertheless, does spheroids really act like liver cells? The question is still being studied. Although spheroids can secrete, form (aggregate), and act as do liver cells, the cells may not be functional because it still undergoes a major environmental change, cultured in vitro. This paper describes how liver cells respond to the different environmental change of being cultured outside the body. It evaluates the liver cells/spheroids morphological formation and functional and biochemical parameters for 21 days. Spheroids grown in culture were compared to in vivo liver cells by measuring spheroid consumption, secretion, and activity.
Primary liver cells were obtained from rats and cultured into spheroids onto plates. Various biochemical assays were ran to compare how spheroids relate to in vivo liver cells. Total protein, glucose, galactose, albumin, pyruvate secretion were determined as well as LDH, g-GT, GPT, and GOT activity. Results were as following: galactose and pyruvate consumption was maintained at a relatively stable level throughout the assay. Glucose secretion and cellular GPT and GOT activities were higher in immature spheroids, then decreased up to maturity and remained stable after. g-GT and LDH activities were initially extremely low and increased as spheroids matured. Albumin secretion decreased rapidly before the formation of the spheroid and increased during maturity. Through the observations made throughout the 21 culture day, the group were able roughtly to divide liver spheroid formation into two days: immaturity (days 1-5) and maturity (> day 5). Throughout spheroid immaturity, the liver cells undergoes a period of biochemical and functional turbulence and after maturity, the spheroid tends to maintain relatively stable functions up to 21 days. As compared to liver cells cultured on monolayers, spheroids are much more related to in vivo liver cells. Nevertheless, it does not imply that spheriods grown in culture can be injected in vivo. Thus, in order to study how liver cells act in vitro, one should develop spheroids and observe them only after maturity, for when they mature, most of their functions have been recovered or maintained at relatively stable levels.
I chose this paper because it relates to the final project in this course. Since, the purpose of the final project can be to propose a method to create a bioartificial liver in a sense, it is crucial to understand the relationship between a liver grown in vitro to one in vivo. I have heard a lot about the importance of spheroids to mimic cells or organs in vivo. Nevertheless, one knows that it is noticeably different for the environment is completely different; the spheroids are grown in a dish. Nevertheless, despite the dramatic difference in environment, this study provides insight about how spheriods are similar and different than a liver. In addition, it gives insight as to parameters and techniques for comparing how well the spheroids mimic the a real liver. For instance, if one wants to observe or test spheroids, one must wait at least 5 days after plating the cells to allow the cells to aggregate and mature. After that, there are a variety of tests that display whether the cells are liver-like or still immature. As in the case for our final project, the amount of production of albumin indicates spheroid maturity and growing liver-like properties.
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Wednesday, November 01, 2006
Functional Tissue Engineering of Articular Cartilage through Dynamic Loading of Chondrocyte-Seeded Agarose Gels
The article can be viewed at http://scitation.aip.org/getabs/servlet/GetabsServlet?prog=normal&id=JBENDY000122000003000252000001&idtype=cvips&gifs=yes
Articular cartilage is limited in its ability to regenerate and to repair as it is not supplied by blood vessels. In spite of the previous efforts in tissue engineering of articular cartilage, current cartilage replacements are only morphologically and biochemically similar to natural cartilage. Their mechanical functionality still needs to be ameliorated for better cartilage substitutes, which is the goal of the authors of this paper. The authors hypothesized that more mechanically functional cartilage can be engineered by subjecting the tissues to dynamic loading at physiological levels.
Three studies were used to test the hypothesis. In the first study, hydrogels made of agarose and alginate at various concentrations without cells were tested for their material properties by a loading device to assess which material is more suitable for use in scaffolds. In the second study, 2% agarose and 2% alginate hydrogels with chondrocytes and acellular controls were cultured without loading. Compositional analysis of sulfated glycosaminoglycan and confined compression testing were carried out for comparison. In the third study, chondrocyte-seeded 2% agarose gels were cultured in two conditions: unconfined compression loading and unloading. Sulfated glycosaminoglycan and hydroxyproline compositional analysis, as well as confined and unconfined stress relaxation testing, were performed at different times.
From the first study, subphysiological peak stresses of agarose gels were observed when they were subjected to physiological cartilage strain levels. The authors found it more reliable to evaluate the aggregate modulus from the equilibrium stress-strain response rather than the transient response. From the second study, the peak equilibrium aggregate modulus measured for the cell-seeded agarose gels was three-fold better than that for cell-seeded alginate gels; moreover, initial increase in sulfated glycosaminoglycan content lasts longer for cell-seeded agarose gels, suggesting that agarose be a better scaffold material. From the third study, the equilibrium modulus of cell-seeded agarose gels with dynamic loading measured at day 28 was 21-fold better than that measured at day 0; under unloading condition, agarose gels only showed a three-fold increase between the same time points. Lastly, the sulfated glycosaminoglycan content of loaded agarose gels remained accumulated at day 21 whereas that of unloaded hydrogels plateaued at day 14.
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Monday, October 30, 2006
Functional small-diameter neovessels created using endothelial progenitor cells expanded ex vivo
View article at: http://www.nature.com/nm/journal/v7/n9/pdf/nm0901-1035.pdf
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The objective of this research is to create small diameter blood vesselswith endothelial progenitor cells (EPCs) that circulate in the blood. EPCs from peripheral blood are an endothelial cell source and typicallymigrate to regions with injured endothelia. What makes EPCs unique is itsability to produce nitric oxide, a vasodilator, and promote patency. Previously, in vitro culture of smooth muscles and endothelial cells onbiodegradable or biological scaffold material were used to produce avessel, but these grafts often times developed thrombosis, aggregation of blood factors that causes vascular obstruction, shortly after implantation.
EPCs were first isolated from blood samples from 1 to 2 week old lambs,cultured ex vivo, and then seeded onto decellularized vascular vesselsprepared from porcine iliac arteries 4 mm in diameter and 4-5 cm inlength. After seeding, grafts were preconditioned with variations ofshear stress in order to achieve maximal retention. The production ofnitric oxide was then assessed using an organ chamber. When exposed tocalcium inonphore A23187, grafts not seeded with EPCs remained contractedwhile grafts seeded with EPCs relaxed. This shows that EPC-seeded graftsproduced nitric oxide. EPC-seeded grafts were then implanted into sheepand data shows that all grafts seeded with EPCs were fully patent 130 daysafter implantation, whereas non-seeded EPC grafts occluded within 15 days. Due to the EPC-seeded grafts’ ability to contract and produce nitricoxide proves that EPCs are ideal in creating small-diameter vessels.
I chose this article because it is relevant and applicable to a large majority of the population since cardiovascular disease continues to be the leading cause of death in the US. It's also valuable to know that studies are being done to provide alternative, non-invasive treatments for cardiovascular disease.
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Autologous Human Tissue-Engineered Heart Valves: Prospects for Systemic Application
To view the article, visit http://gateway.ut.ovid.com/gw1/ovidweb.cgi and type in the above title.
Past efforts on heart valve replacement have concentrated on the development of pulmonary (to the lungs) rather than systemic valves and the resultant valves have also proved unable to properly grow, adapt, and heal. In their July 2006 article, Anita et al. successfully incorporated several recently published techniques of cell seeding using fibrin gel (as a cell carrier), cell culture on a biodegradable scaffold, and mechanical cell conditioning to induce more anisotropy and valve-like behavior. Cells simply cultured statically were compared with cells subject mechanical conditioning in a bioreactor that simulates blood flow in a human heart, especially during diastole (when the heart dilates as it is filled with blood).
The original cells were harvested from the vena saphena magma of a 77 year old man and then isolated using an automated cell staining system and three primary antibodies. The trileaflet heart valves were grown into the correct shape using a mold, stents to hold up each leaflet, and scaffolds that had been sterilized with 70% ethanol. These cells were allowed to grow with media which among other components, contained 10% fetal bovine serum. Cells were than either a.)simply left to grow on culture flasks, b.) simply left to grow in the aforementioned bioreactor, and c.) grown in the bioreactor mimicking the heart’s diastolic phase with pressure differences of 5 to 30 mm Hg. The cells in group c.) were analyzed after 2, 4, and 6 weeks while the a.) and b.) cells were analyzed at the 4 week mark only.
While the conditioning proved to have little effect on cell growth or collagen content, it did succeed in generating tissue with more uniform mechanical properties than the statically grown controls. While the tissue engineered valves were able to generate similar stress strain curves in the radial direction as compared real heart valves, they performed less strongly in the circumferential direction. This most likely contributed to a larger problem - the valves opened correctly but failed to close completely, allowing blood to flow in the opposite direction. While further efforts must obviously be made in perfecting this technique, this new method of valve replacement culture shows great promise.
I first chose this article for its creative application of recent advances to tailor and design a new way to create a sorely needed tissue engineered device; reading widely and applying previously proven results to our project design is something we could all come into the habit of doing as engineers. The methods of tissue culture and testing were too numerous to mention completely, but this article is a great example of a large scale combination of various analytic tools we have learned about in class including histology, recognition using antibodies, mechanical stress/strain testing, cell counting by dyes to determine DNA amount (similar to our technique of nuclear staining with DAPI).
(Terry sez: a direct link to the paper can be found here - http://circ.ahajournals.org/cgi/content/full/114/1_suppl/I-152)
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Sunday, October 29, 2006
Tissue engineered cartilage: Utilization of autologous serum and serum-free media for chondrocyte culture
The main focus of this study is to examine the possible use of autologous serum and serum free media in chondrocyte growth for tissue engineered cartilage. They focus on the the different rates of proliferation of chondrocytes between the media with autologous serum, serum free media and the media with standard fetal bovine serum (FBS).
Chondrocytes were first isolated by taking auricular cartilage from pigs and fragmenting the sample. The sample was then washed, digested with 0.3% collagenase II, and filtered. The filtrate was taken and cell pelleted for use in the experiment. The chondrocytes were plated and the sample was placed into three different flasks with equal concentrations. The chondrocytes were subjected to three different media: Ham F12 culture media with 10% FBS, Ham F12 culture media with 10% autologous serum and Ham F12 culture media with growth factors. The culture was changed twice a week with morphology examined using light microscopy. The cells were trypsinized at days 3, 6, 9, and 12 with 0.25% Trysin/EDTA and counted with a hematocytometer.
The results showed that while the cells in the media with FBS grew faster initially, the cells in the serum-free media eventually caught up to the same cell count while the cells in the media with autologous serum grew at a slower rate. These findings prove that it is possible for chondrocyte expansion using media with autologous serum and serum-free media. The potential of these results is that the use of different media could reduce possible immunological reactions or vector infections from the FBS.
I chose this paper due to the similarities with our current labs involving Rex and 3T3 cells. In our lab we determined that the calf serum we were using was possibly influencing our results by containing some proteins that were analyzed in our quantification of protein. By using the serum-free media we could have nullified the serum's effects. Also, this directly applies to our goals of TE cartilage. Lastly, I feel that this paper illustrates various techniques we learned in class such as passaging and cell counting.
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Saturday, October 28, 2006
Tissue-Engineered Human Vascular Media Produced in Vitro by the Self-Assembly Approach Present Functional Properties Similar to Those of Their Native Blood Vessels
See the full text in http://www.liebertonline.com/doi/abs/10.1089/ten.2006.12.2275
The main object for their research is to develop vascular models which can be use for experimental studies in vitro. They are focusing on reconstruct the tissue-engineered vascular media, which is a very good in vitro model for the study of the functionality of human blood vessels.
The way to do this is first obtaining the endothelial cells from human umbilical vein. They test the responds of the human umbilical veins to endothelial cells(ET), and they figure out that by the activation of the ET receptors, the veins are able to responses to the ET. They then use the vascular smooth muscle cell to reconstruct the tissue-engineered vascular media. They first isolated the smooth muscle cell from the umbilical cord veins, and then culture the cell from human umbilical cord veins which has the expression on both the ET receptors. Then the smooth muscle cells are used to reconstruct the cultured media. By using the RT-PCR, they find out that there is mRNA of the both the ET receptors inside the Media they just reconstructed. By comparing the result with other publishes, the media shows the similar response to ET as the blood vessel from the smooth muscle cells.
Human blood vessels have very complex structures and they are not easy to take care. Therefore, doing experiments on human blood vessels to study the blood vessel functionality are like impossible work. For this reason, people want to use models rather than using the real blood vessels to the relative research. I like this article, because it gives idea on the development of blood vessels model. They can reconstruct the vascular media by using the tissue-engineered methods: isolates the vascular smooth muscle cells from human umbilical cord veins. They also test the response of the vascular media to blood vascular cells, and confirm that the media have similar kinds of response as the regular blood vessel.
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Friday, October 27, 2006
http://www3.interscience.wiley.com/cgi-bin/fulltext/113391970/HTMLSTART
Growing tissue-like constructs with Hep3B/HepG2 liver cells on PHBV microspheres of different sizes
In this paper, the researchers were interested in the molecular, functional, and proliferative behaviors of liver cells, from the Hep3B and HepG2 hepatoma cell lines, seeded on 8% poly[3-hydroxybutyrate-co-3-hydroxyvalerate] (PHBV) microspheres as compared to the liver cells cultured 2-dimentionally with laminin and poly-L-lysine (positive control). This new cell seeding technique could become a possible cell growing methods in a tissue engineered liver/liver device. They choose PHBV because it is biocompatible, biodegradable, and non-cytotoxic in vivo. The microspheres were made by emulsifying and homogenizing 8% PHBV oil-in-water-in-oil solution, followed by evaporation of the solvent. The researchers considered microsphere size as a parameter and made 3 different sizes of microsphere by changing the homogenizer’s speed. After the microspheres were made, hepatoma cells were seeded onto them and cultured. As positive control, hepatoma cells are cultured two dimensionally with laminin and poly-L-lysine. Polyurethane film with zinc diethydithiocarbamate was used as negative control. At the appropriate time points, the cultured is analyzed. The analysis includes MTT assay for viability, bisbenzimide fluorescent assay for cell proliferation, ELISA assay to quantify albumin (since healthy liver cells make albumin), and EROD assay to test cytochrome P-405 activity (which measure liver cell’s detoxification activity).
The researchers were able to show that cells cultured on the microsphere spread over the microsphere and connect the adjacent microspheres together. There were multiple cells layer formed in the space between the microspheres. More interesting, it was shown that cells seeded on the microsphere had higher proliferation rate and viability, secreted more albumin, and had higher detoxification (cytochrome P-405) activity than the positive control. This means that the cells are able to live longer, divide better, and maintain liver specific activities/functions better. These behaviors of cells cultured on microsphere made this new culturing method a good choice to use in a tissue-engineered liver or liver device.
The reasons I chose the paper are as followed. (1) Liver is a very important organ and many people are waiting for the limited liver transplantation. This paper is attempting to solve this problem by researching tissue engineered liver. (2) Many of the finding in this paper will be useful for a tissue engineered (TE) liver. For example, liver cells grow on microsphere proliferate better and have higher viability. This is extremely important since primary cells used in TE liver are limited, usually not very proliferative, and their viability decrease with time. This new technique could improve, if not solve, these problems. Livers cells seeded on the microsphere secreted higher albumin and have higher P-405 activity, suggesting that they maintain their function and not likely to de-differentiate. This aspect is especially useful in TE liver since we want the cells to maintain their function instead of ceasing to act like liver cells. (3) I think it’s really nice that this paper use many of the methods we learned in class such as trypan blue plus other live/dead assay, and ELISA. I picked this paper because the materials are relevant to the class and tissue engineering.
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Thursday, October 26, 2006
Autologous full-thickness skin substitute for healing chronic wounds
The paper’s objective was to develop tissue engineered skin with human origin in order to use to heal wounds. The paper focused on the development of skin in order to heal ulcers. To develop the tissue engineered skin, the investigators harvested a 3-mm biopsy from the patient’s leg. From this sample of human skin, they prepared an acellular human allodermis. Dermal fibroblasts were cultured along with epidermal sheets. The next step was placing epidermal sheets stratum corneum side up onto the allodermis and then culturned in keratinocyte medium for approximately 7 days. The allodermis with the epidermal sheets were then placed on the fibroblasts to allow for migration. With further culturing and addition of growth factors, antibiotics, and growth medium, the tissue engineered skin was ready in three weeks. Within the three week period the epidermis expanded to cover to allordermis, with a surface area of 1.5 cm2 from the original 3-mm biopsy. Like human skin, the engineered skin was comprised of a compact basal layer, spinous layer, granular layer, and statum corneum.
The engineered skin was applied to the skin using Lomateull® H and providone-iodine ointment. The engineered skin was used to treat nineteen ulcers in fourteen patients. The use of engineered skin resulted in pain reduction from the ulcers. Within one week of application, the engineered skin expanded to the surrounding skin of the ulcer. In twelve of the nineteen ulcers, the engineered skin was incorporated into the wound. The median time for healing was 6 weeks. However, in seven of the nineteen ulcers, the skin was not incorporated and could be removed from the wound.
I choose this paper because it demonstrates the effectiveness of using tissue engineered skin in order to treat wounds. This paper shows that a small sample of human skin can be used to create an effective treatment. Tissue engineered skin is an important area of research and development to help the myriad of skin conditions and also treating severe damage, like burns. Although three weeks is a long time to develop the skin, it is a great alternative to skin grafts where a large area of healthy skin is needed.
Gibbs, S., van den Hoogenband, H.M., Kirtschig, G., Richters, C.D., Spiekstra, S.W., Breetveld, M., Scheper, R.J., and de Boer, E.M. “Autologous full-thickness skin substitute for healing chronic wounds.” British Journal of Dermatology 155 (2006): 267-274.
PubMed Link:
Click Here
Full Text Link (UC-elinks):
http://www.blackwell-synergy.com/doi/abs/10.1111/j.1365-2133.2006.07266.x
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Monday, September 18, 2006
To get the ball rolling, let's take a peek at Synthetic biomaterials as instructive extracellular microenvironments for morphogenesis in tissue engineering.
This paper is interested in how synthetic biomaterials can deliver soluble (growth factor-like) and insoluble (extracellular matrix-like) signals to cells seeded into or in the viscinity of the biomaterial. This signaling influences cell processes, and the resulting migration, proliferation, differentiation, etc. will determine cell fate and the functionality of the tissue engineered device.
This is a review paper, and thus not bad at giving you an idea of what's been done and suggesting (largely in figures 2 and 4) potential design principles. Consider how you might use this paper to inform the "future work" section of your project write-ups.
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