Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells

Gastric cancer is a significant health threat. The resistance to conventional treatments and recurrence has been associated with the presence of a population of cells within the tumour, known as cancer stem cells (CSCs). It was proposed that specifically targeting the CSCs may be an efficacious canc...

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Main Author: Tan Mei Qi
Other Authors: Tan Lay Poh
Format: Final Year Project
Language:English
Published: 2016
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Online Access:http://hdl.handle.net/10356/66702
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Institution: Nanyang Technological University
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spelling sg-ntu-dr.10356-667022023-03-04T15:30:31Z Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells Tan Mei Qi Tan Lay Poh School of Materials Science and Engineering DRNTU::Engineering Gastric cancer is a significant health threat. The resistance to conventional treatments and recurrence has been associated with the presence of a population of cells within the tumour, known as cancer stem cells (CSCs). It was proposed that specifically targeting the CSCs may be an efficacious cancer therapy, hence driving many ongoing researches to enrich CSCs to support the understanding of cancer as well as the development of targeted treatment. In this report, 3D electrospun PLGA scaffold was fabricated to investigate the proliferation and differentiation of gastric cancer MKN28 cells encapsulated in gelatin methacrylate (GelMA). Characterization of the scaffold including properties such as fibre morphology and diameter, pore size and porosity, as well as mechanical properties, was done. Expression of genes was studied using quantitative polymerase chain reaction. Upregulation of Oct4A and Sox2 indicated that cells might have differentiated to obtain stem-like characteristics, however downregulation of CD44 suggested that identification of presence of CSCs needs to be further investigated using more markers. As many had reported a correlation between CSCs and EMT, EMT was also studied to demonstrate any possible relationship. Upregulation of Snail1, Twist1, Twist2 and Zeb1 could have induced an EMT by repressing E-cadherin, as shown in the E-cadherin downregulation after day 3. However, the upregulation of E-cadherin after day 7 could not be explained at this stage. In addition, absence of N-cadherin and vimentin expression indicated that EMT might be in its initial stages. These findings necessitate further studies to validate if EMT was induced. The higher genes expression but lower proliferation of cells in hybrid sample as compared to pure scaffold pointed out that the scaffold will provide a suitable platform for further studies to optimise the hybrid sample to be used as a microenvironment to enrich CSCs. Bachelor of Engineering (Materials Engineering) 2016-04-21T06:30:17Z 2016-04-21T06:30:17Z 2016 Final Year Project (FYP) http://hdl.handle.net/10356/66702 en Nanyang Technological University 34 p. application/pdf
institution Nanyang Technological University
building NTU Library
continent Asia
country Singapore
Singapore
content_provider NTU Library
collection DR-NTU
language English
topic DRNTU::Engineering
spellingShingle DRNTU::Engineering
Tan Mei Qi
Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells
description Gastric cancer is a significant health threat. The resistance to conventional treatments and recurrence has been associated with the presence of a population of cells within the tumour, known as cancer stem cells (CSCs). It was proposed that specifically targeting the CSCs may be an efficacious cancer therapy, hence driving many ongoing researches to enrich CSCs to support the understanding of cancer as well as the development of targeted treatment. In this report, 3D electrospun PLGA scaffold was fabricated to investigate the proliferation and differentiation of gastric cancer MKN28 cells encapsulated in gelatin methacrylate (GelMA). Characterization of the scaffold including properties such as fibre morphology and diameter, pore size and porosity, as well as mechanical properties, was done. Expression of genes was studied using quantitative polymerase chain reaction. Upregulation of Oct4A and Sox2 indicated that cells might have differentiated to obtain stem-like characteristics, however downregulation of CD44 suggested that identification of presence of CSCs needs to be further investigated using more markers. As many had reported a correlation between CSCs and EMT, EMT was also studied to demonstrate any possible relationship. Upregulation of Snail1, Twist1, Twist2 and Zeb1 could have induced an EMT by repressing E-cadherin, as shown in the E-cadherin downregulation after day 3. However, the upregulation of E-cadherin after day 7 could not be explained at this stage. In addition, absence of N-cadherin and vimentin expression indicated that EMT might be in its initial stages. These findings necessitate further studies to validate if EMT was induced. The higher genes expression but lower proliferation of cells in hybrid sample as compared to pure scaffold pointed out that the scaffold will provide a suitable platform for further studies to optimise the hybrid sample to be used as a microenvironment to enrich CSCs.
author2 Tan Lay Poh
author_facet Tan Lay Poh
Tan Mei Qi
format Final Year Project
author Tan Mei Qi
author_sort Tan Mei Qi
title Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells
title_short Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells
title_full Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells
title_fullStr Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells
title_full_unstemmed Role of 3D electrospun PLGA scaffold on proliferation and differentiation of gastric cancer cells
title_sort role of 3d electrospun plga scaffold on proliferation and differentiation of gastric cancer cells
publishDate 2016
url http://hdl.handle.net/10356/66702
_version_ 1759855456901136384