Organotypic keratinocyte cultures on de-epithelialized tongue mucosa
Organotypic cultures have been used to study epithelial cell behavior for many years. The aim of this study was to develop an organotypic culture method that better mimics the three-dimensional morphology of interdigitating rete ridges and connective tissue (CT) papillae and conserves the basemen...
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2009
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ndltd-UBC-oai-circle.library.ubc.ca-2429-106342018-01-05T17:35:24Z Organotypic keratinocyte cultures on de-epithelialized tongue mucosa Hildebrand, H. Christopher Organotypic cultures have been used to study epithelial cell behavior for many years. The aim of this study was to develop an organotypic culture method that better mimics the three-dimensional morphology of interdigitating rete ridges and connective tissue (CT) papillae and conserves the basement membrane zone (BMZ). Bovine tongue mucosa was chosen for the raft donor and incubated with cold 1 M sodium chloride solutions for 4 days to separate the epithelial tissue from the BMZ and underlying CT matrix. Level of separation was studied by electron microscopy (EM) and immunohistochemical staining of several integrin subunits, laminin-1 and -5, type IV and Vll collagen, tenascin, fibronectin, vitronectin and heparan sulfate proteoglycan. After the separation, IHC staining and EM observations suggest a separation through the lamina lucida. Rafts were used for growth of organotypic cultures of human keratinocytes. Three different keratinocyte cell lines were cultured submerged for 6 days after which the cultures were raised to air-liquid interface and maintained for up to 40 days. Sections were prepared for routine histology, EM and IHC staining. Histomorphology varied significantly between the cell lines. Sometimes more than 15 cell layers resembling normal epithelial histology were present. Keratinocytes in these raft cultures were found to express P4 integrins against the preexisting BMZ. In addition, human keratinocytes deposited their own matrix molecules, particularly tenascin, laminin-1 and -5. Expression of integrin subunits and differentiation markers revealed some differences from normal tissue, which depended on the cell line. The ultrastructure of the BMZ including hemidesmosomes was similar to the normal dermal-epidermal junction. This culture model seems to mimic normal epithelium including the BMZ and is potentially useful for multiple applications for studies on epithelial cell behavior in vitro. Dentistry, Faculty of Graduate 2009-07-10T22:33:31Z 2009-07-10T22:33:31Z 2000 2000-11 Text Thesis/Dissertation http://hdl.handle.net/2429/10634 eng For non-commercial purposes only, such as research, private study and education. Additional conditions apply, see Terms of Use https://open.library.ubc.ca/terms_of_use. 5505369 bytes application/pdf |
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NDLTD |
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English |
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Others
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NDLTD |
| description |
Organotypic cultures have been used to study epithelial cell behavior for many
years. The aim of this study was to develop an organotypic culture method that
better mimics the three-dimensional morphology of interdigitating rete ridges and
connective tissue (CT) papillae and conserves the basement membrane zone
(BMZ).
Bovine tongue mucosa was chosen for the raft donor and incubated with cold 1 M
sodium chloride solutions for 4 days to separate the epithelial tissue from the BMZ
and underlying CT matrix. Level of separation was studied by electron microscopy
(EM) and immunohistochemical staining of several integrin subunits, laminin-1 and
-5, type IV and Vll collagen, tenascin, fibronectin, vitronectin and heparan sulfate
proteoglycan. After the separation, IHC staining and EM observations suggest a
separation through the lamina lucida. Rafts were used for growth of organotypic
cultures of human keratinocytes. Three different keratinocyte cell lines were
cultured submerged for 6 days after which the cultures were raised to air-liquid
interface and maintained for up to 40 days. Sections were prepared for routine
histology, EM and IHC staining. Histomorphology varied significantly between the
cell lines. Sometimes more than 15 cell layers resembling normal epithelial
histology were present. Keratinocytes in these raft cultures were found to express
P4 integrins against the preexisting BMZ. In addition, human keratinocytes
deposited their own matrix molecules, particularly tenascin, laminin-1 and -5.
Expression of integrin subunits and differentiation markers revealed some
differences from normal tissue, which depended on the cell line. The ultrastructure
of the BMZ including hemidesmosomes was similar to the normal dermal-epidermal
junction. This culture model seems to mimic normal epithelium including the BMZ
and is potentially useful for multiple applications for studies on epithelial cell
behavior in vitro. === Dentistry, Faculty of === Graduate |
| author |
Hildebrand, H. Christopher |
| spellingShingle |
Hildebrand, H. Christopher Organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| author_facet |
Hildebrand, H. Christopher |
| author_sort |
Hildebrand, H. Christopher |
| title |
Organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| title_short |
Organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| title_full |
Organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| title_fullStr |
Organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| title_full_unstemmed |
Organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| title_sort |
organotypic keratinocyte cultures on de-epithelialized tongue mucosa |
| publishDate |
2009 |
| url |
http://hdl.handle.net/2429/10634 |
| work_keys_str_mv |
AT hildebrandhchristopher organotypickeratinocyteculturesondeepithelializedtonguemucosa |
| _version_ |
1718588613332041728 |