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Decellularization for the Preparation of Highly Preserved Human Acellular Skin Matrix for Regenerative Medicine
* These authors contributed equally
In This Article
Summary
Decellularized human skin is suitable for tissue regeneration. A major issue of decellularization is the preservation of the native architecture, along with the appropriate content of structural proteins, glycosaminoglycans (GAGs), and growth factors. The method proposed allows fast and effective decellularization, producing decellularized skin with well-preserved native features.
Abstract
Extracellular matrix (ECM) provides biophysical and biochemical stimuli to support self-renewal, proliferation, survival, and differentiation of surrounding cells due to its content of diverse bioactive molecules. Due to these characteristics, the ECM has been recently considered a promising candidate for the creation of biological scaffolds to boost tissue regeneration. Emerging studies have demonstrated that decellularized human tissues could resemble the native ECM in their structural and biochemical profiles, preserving the three-dimensional (3D) architecture and the content of fundamental biological molecules. Hence, decellularized ECM can be employed to promote tissue remodeling, repair, and functional reconstruction of many organs. Selecting the appropriate decellularization procedure is crucial to obtain acellular tissues that retain the characteristics of the ideal microenvironment for cells.
The protocol described here provides a detailed step-by-step description of the decellularization method to obtain a reproducible and effective cell-free biological ECM. Skin fragments from patients undergoing plastic surgery were scaled down and decellularized using a combination of sodium dodecylsulfate (SDS), Triton X-100, and antibiotics. To promote the regular and homogeneous transport of the solution through the samples, they were enclosed in embedding cassettes to ensure protection from mechanical insults. After the decellularization procedure, the snow-white color of skin fragments indicated complete and successful decellularization. Additionally, decellularized samples showed an intact and well-preserved architecture. The results suggest that the proposed decellularization method was effective, fast, and reproducible and protected samples from architectural damages.
Introduction
The ECM serves as a scaffold for cells, supporting them through an intricate architecture maintained by different components, and it is one of the major factors responsible for the mechanical properties of the heart and cardiac tissue function1,2. Increasing evidence suggests that ECM plays an active role in tissue remodeling, making the conventional assumption that the ECM is a passive component obsolete3,4,5,6. The role of the ECM is to provide biophysical and biochemical cues to ....
Protocol
The specimens from human tissue were collected according to the principles of the Declaration of Helsinki and observing University Hospital "Federico II" guidelines. All patients involved in this study provided written consent forms.
1. Preparation of solutions
- Preparation of 1200 mL of 1% decellularizing solution
- Prepare 600 mL of 2% Triton X-100 solution by measuring 588 mL of double-distilled water in a graduated cylinder and transferring it to a 1 L beaker. .......
Representative Results
The aim of the protocol was to obtain a skin d-ECM sample from biological tissue, maintaining a well-organized 3D structure and well-preserved content of biological molecules (Figure 1). This method is primarily based on the constant stirring of the samples in a solution containing the combination of two detergents, Triton X-100 and SDS, thus preserving the biological and structural features typical of the native tissue and reducing the time of exposure during the decellularization process. .......
Discussion
Although the protocol described above has been optimized and improved compared to previously published protocols, it presents a few critical steps that need attention and precision. The formation of foam must be avoided during the preparation of the decellularizing solution to prevent incorrect dilution of the detergents. This could be addressed by gently pouring the solutions and making them flow along the inner side of the cylinder. Furthermore, care must be taken when manually removing fat tissue from the samples, as .......
Acknowledgements
None
....Materials
| Name | Company | Catalog Number | Comments |
| 0.9% NaCl isotonic Physiological solution | Sigma-Aldrich | S8776 | 0.9% in water |
| 1 L beaker | VWR | 511-0318 | Clean and autoclave before use |
| 10 mL serological pipet | Falcon | 357551 | Sterile, polystyrene |
| 100 mm plates | Falcon | 351029 | Treated, sterile cell culture dish |
| 15 mL sterile tubes | Falcon | 352097 | Centrifuge sterile tubes, polypropylene |
| 1 L graduated cylinder | VWR | 612-1524 | Clean and autoclave before use |
| 2 L bottle | VWR | 215-1596 | Clean and autoclave before use |
| 25 mL serological pipet | Falcon | 357525 | Sterile, polystyrene |
| 2 L graduated cylinder | VWR | 612-3072 | Clean and autoclave before use |
| 500 mL beaker | VWR | 511-0317 | Clean and autoclave before use |
| Amphotericin B | Sigma-Aldrich | Y0000005 | Powder |
| Dissecting board | VWR | 100498-398 | Made of high-density polyethylene. |
| Dissecting scalpel | VWR | 233-5526 | Sterile and disposable |
| Embedding cassettes | Diapath | 070191 | External dimensions: 40x26x7 mm (WxDxH) |
| Fine forceps | VWR | 232-1317 | Clean and autoclave before use |
| Funnel | VWR | 221-1861 | Clean and autoclave before use |
| Hexagonal weighing boats size M | Sigma-Aldrich | Z708585 | Hexagonal, polystyrene, 51 mm Bottom I.D., 64 mm Top I.D. |
| Hexagonal weighing boats size S | Sigma-Aldrich | Z708577 | Hexagonal, polystyrene, 25 mm Bottom I.D., 38 mm Top I.D. |
| Large surgical scissors | VWR | 233-1211 | Clean and autoclave before use |
| Long forceps | VWR | 232-0096 | Clean and autoclave before use |
| Penicillin and Streptomycin | Sigma-Aldrich | P4333-100ml | Stabilized, with 10.000 units penicillin and 10 mg streptomycin/mL, 0.1 μm filtered. Store at -20°C. The solution should be aliquoted into smaller working volumes to avoid repeated freeze/thaw cycles Solution. |
| Pipette gun | Eppendorf | 613-2795 | Eppendorf Easypet® 3 |
| Plastic tray | VWR | BELAH162620000 | Corrosion-proof polypropylene plastic tray |
| Potassium Chloride | Sigma-Aldrich | P9333 | Powder |
| Potassium Phosphate Monobasic | Sigma-Aldrich | P5665 | Powder |
| Sodium Chloride | Sigma-Aldrich | S7653 | Powder |
| Sodium Dodecyl Sulfate | Sigma-Aldrich | 62862 | Powder |
| Sodium Phosphate Dibasic | Sigma-Aldrich | 94046 | Powder |
| Spatula | VWR | RSGA038.210 | Clean and autoclave before use |
| Spoon | VWR | 231-1314 | Clean and autoclave before use |
| Stir bar | VWR | 442-0362 | Clean and autoclave before use |
| Stir bar retriever | VWR | 89026-262 | Molded in pure, FDA-approved PTFE |
| Triton X-100 | Sigma-Aldrich | 9002-93-1 | Liquid |
References
- Daley, W. P., Peters, S. B., Larsen, M. Extracellular matrix dynamics in development and regenerative medicine. Journal of Cell Science. 121 (3), 255-264 (2008).
- Lu, P., Takai, K., Weaver, V. M., Werb, Z. Ex....
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