Table 3.
Biomolecules used for tympanic membrane regeneration by tissue engineering.
| Biomolecule | Properties | Model | Main findings |
|---|---|---|---|
| EGFl9,48-52 | Mitogenic effect | Animal | Greater tympanic closure in less time Neomembrane thickness and histology similar to the native membrane; the thickness achieved in spontaneous closure is less than half the normal thickness of the TM Stimulated neovascularization and fibroblast number Stimulated proliferation (mainly of the squamous layer) Long-term application leads to re-perforation and cholesteatoma formation |
| Human | No improvement of tympanic closure No toxicity |
||
| TGF-α53,54,60 | In vitro | More effective than EGF in promoting colony dispersion and injuries healing Greater pro motility activity than EGF |
|
| Animal | TGF-α was not observed in normal TM, but it was expressed after a perforation | ||
| TGF-β65 | Chemotaxis induction Extracellular matrix production Angiogenesis stimulation Possible excess of scar tissue Thicker TM |
Animal | Reduction of perforation closure time Need to repeated application to achieve the above beneficial effects Possible formation of a disorganized fibrous scar |
| PGF45,46,55-59 | Stimulation of fibroblast, endothelial cells and keratinocytes proliferation and differentiation Stimulation of collagen fibrils growth Vasodilation promoting Stimulation of protease production |
Animal | Epithelial and/or connective tissue hiperplasia Increased success of tympanic closure when applied directly to the perforation; if applied with Gelfoam®, it forms a voluminous scar that protrudes from the middle ear cavity and ossicles (use of Gelfoam® inadvisable) |
| Human | Increased tympanic closure rate and reduced time of TM closure Enhanced hearing recovery Possible epithelial pearl formation Reduction of middle ear infections Hyperplasia of granulation tissue - which disappears in 5-7 days |
||
| KGF60,61 | Reactive oxygen species detoxyfication Promotion of re-epithelialization Keratinocytes proliferation and migration |
Animal | Enhanced epithelial migration and proliferation in the first steps No increase in tympanic closure rate More organized repair process |
| PDGF62,63 | Fibroblast mitogen | Animal | Increased tympanic closure rate Reduction of perforation closure time More abundant connective fibrous tissue layer |
| Human | No increase in tympanic closure | ||
| VEGF64 | Fibroblast mitogen Angiogenesis stimulation Induction of collagen deposition Induction of epithelialization |
Animal | VEGF is more specific and important than bFGF in acute perforation closure |
| Autologous serum from peripheral blood21 | Promotion of wound healing Lack of antigenicity Large quantity of growth factors |
Human | ASET does not require anesthesia, reduces or completely closes chronic perforations and implies a continuous supply of growth factors by the own patient Further studies are required to conclude whether the beneficial effect is due to the serum or to the scaffold used for the tympanic membrane closure |
| Human umbilical cord serum68 | Large quantity of growth factors (greater concentration of EGF, NGF and TGF-αβ than in autologous serum from peripheral blood) | Animal | Applied with a 3D collagen scaffold, it enhances significantly chronic perforation closure and hearing capacity from early stages than with paper patches Neomembrane thickness similar to the native membrane Further studies are required to conclude whether the beneficial effect is due to the serum or to the scaffold used for the tympanic membrane closure |
| Hyaluronic acid19,69 | Viscoelastic properties It can be used as a scaffold or as a biomolecule administered in drops Increased motility and phagocytic activity of polimorfonuclear leucocytes |
Animal | Reduced time in tympanic perforation closure Increased closure success rate than natural closure Increased levels of FGF and VEGF |
| Human | No increased tympanic closure success rate | ||
| Human insulin66,70 | Neovascularization Increased fibroblast growth rate Increased keratinocytes proliferation, migration and differentiation from the perforation edges Activation of insulin receptor and IGF 1 receptor |
Animal | Beneficial effect in perforation epithelialization Neovascularization Formation of finger-like projections Fibroblast activity Presence of inflammatory cells in the lamina propria |
| Stimulation of keratyn migration | Human | Increased micro-vascularization from the remnants of tympanic membrane or graft towards the perforation, with the induction of inflammation and epithelialization from the perforation edges Halfen the perforation size after its forth or fifth application |
|
| Platelet-rich plasma67 | α granules of platelets contain growth factors | Animal | Reduction of the average time of tympanic closure |
| Plasminogen71,72 | Degradation of fibrin and extracellular matrix proteins | Animal | Reduced time of tympanic closure |
EGF, epidermic growth factor; TM, tympanic membrane; TGF-α, -β, transformant growth factor type α, -β; FGF, fibroblast growth factor; KGF, keratinocyte growth factor; PDGF, platelet-derived growth factor; VEGF, vascular endothelial growth factor; bFGF, basic fibroblast growth factor; ASET, autologous serum eardrop therapy; NGF, nerve growth factor; IGF-1, insulin-like growth factor type I.