Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions

Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions

Parvathy Venugopal1, Sudha Balasubramanian1, Anish Sen Majumdar1, Malancha Ta21Stempeutics Research Pvt. Ltd, Manipal Hospital, Bangalore, India; 2Manipal Institute of Regenerative Medicine, Manipal University, Bangalore, IndiaAbstract: Mesenchymal stem cells (MSCs) have become an attractive tool fo...

Descripción completa

Guardado en:
Detalles Bibliográficos
Autores principales: Venugopal P, Balasubramanian S, Sen Majumdar A, Ta M
Formato: article
Lenguaje:EN
Publicado: Dove Medical Press 2011
Materias:
Cytology
QH573-671
Acceso en línea:https://doaj.org/article/dc46bda55d9745d2bd2e4eb812b602ba
Etiquetas: Agregar Etiqueta
Sin Etiquetas, Sea el primero en etiquetar este registro!
id oai:doaj.org-article:dc46bda55d9745d2bd2e4eb812b602ba
record_format dspace
spelling oai:doaj.org-article:dc46bda55d9745d2bd2e4eb812b602ba2021-12-02T01:31:56ZIsolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions1178-6957https://doaj.org/article/dc46bda55d9745d2bd2e4eb812b602ba2011-04-01T00:00:00Zhttp://www.dovepress.com/isolation-characterization-and-gene-expression-analysis-of-whartonrsqu-a7203https://doaj.org/toc/1178-6957Parvathy Venugopal1, Sudha Balasubramanian1, Anish Sen Majumdar1, Malancha Ta21Stempeutics Research Pvt. Ltd, Manipal Hospital, Bangalore, India; 2Manipal Institute of Regenerative Medicine, Manipal University, Bangalore, IndiaAbstract: Mesenchymal stem cells (MSCs) have become an attractive tool for tissue engineering and targets in clinical transplantation due to their regeneration potential and immuno-suppressive capacity. Although MSCs derived from bone marrow are the most widely used, their harvest requires an invasive procedure. The umbilical cord, which is discarded at birth, can provide an inexhaustible source of stem cells for therapy. The Wharton’s jelly-derived MSCs (WJ-MSCs), from the umbilical cord, have been shown to have faster proliferation rates and greater expansion capability compared with adult MSCs. The standard isolation and in vitro culture protocol for WJ-MSCs utilizes fetal bovine serum (FBS) or calf serum as a nutrient supplement. However, FBS raises potential safety concerns such as transmission of viral/prion disease and may initiate xenogeneic immune reactions against bovine antigens. Therefore, for therapeutic applications, there is an urgent requirement to establish an alternative nutrient supplement which would favor cell proliferation, retain MSC characteristics, and prove safe in human subjects. In the present study, we isolated and expanded WJ-MSCs in 5% pooled, allogeneic human serum (HS) supplemented with 2 ng/mL of basic fibroblast growth factor. For cell dissociation, porcine trypsin was replaced with TrypLE, a recombinant enzyme, and a protease-free protocol was adapted for isolation of MSCs from WJ. We determined their growth kinetics, in vitro differentiation potential, surface marker expression, and colony-forming unit potential and compared them against standard WJ-MSC cultures expanded in 10% FBS. All these parameters matched quite well between the two MSC populations. To test whether there is any alteration in gene expression on switching from FBS to HS, we analyzed a panel of stem cell and early lineage markers using Taqman® low density array. No significant deviation in gene expression was observed between the two populations. Thus we established an efficient, complete xeno-free protocol forpropagation of human WJ-MSCs.Keywords: human serum, explant, trypLE, umbilical cord, FBS, bFGF Venugopal PBalasubramanian SSen Majumdar ATa MDove Medical PressarticleCytologyQH573-671ENStem Cells and Cloning: Advances and Applications, Vol 2011, Iss default, Pp 39-50 (2011)
institution DOAJ
collection DOAJ
language EN
topic Cytology
QH573-671
spellingShingle Cytology
QH573-671
Venugopal P
Balasubramanian S
Sen Majumdar A
Ta M
Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
description Parvathy Venugopal1, Sudha Balasubramanian1, Anish Sen Majumdar1, Malancha Ta21Stempeutics Research Pvt. Ltd, Manipal Hospital, Bangalore, India; 2Manipal Institute of Regenerative Medicine, Manipal University, Bangalore, IndiaAbstract: Mesenchymal stem cells (MSCs) have become an attractive tool for tissue engineering and targets in clinical transplantation due to their regeneration potential and immuno-suppressive capacity. Although MSCs derived from bone marrow are the most widely used, their harvest requires an invasive procedure. The umbilical cord, which is discarded at birth, can provide an inexhaustible source of stem cells for therapy. The Wharton’s jelly-derived MSCs (WJ-MSCs), from the umbilical cord, have been shown to have faster proliferation rates and greater expansion capability compared with adult MSCs. The standard isolation and in vitro culture protocol for WJ-MSCs utilizes fetal bovine serum (FBS) or calf serum as a nutrient supplement. However, FBS raises potential safety concerns such as transmission of viral/prion disease and may initiate xenogeneic immune reactions against bovine antigens. Therefore, for therapeutic applications, there is an urgent requirement to establish an alternative nutrient supplement which would favor cell proliferation, retain MSC characteristics, and prove safe in human subjects. In the present study, we isolated and expanded WJ-MSCs in 5% pooled, allogeneic human serum (HS) supplemented with 2 ng/mL of basic fibroblast growth factor. For cell dissociation, porcine trypsin was replaced with TrypLE, a recombinant enzyme, and a protease-free protocol was adapted for isolation of MSCs from WJ. We determined their growth kinetics, in vitro differentiation potential, surface marker expression, and colony-forming unit potential and compared them against standard WJ-MSC cultures expanded in 10% FBS. All these parameters matched quite well between the two MSC populations. To test whether there is any alteration in gene expression on switching from FBS to HS, we analyzed a panel of stem cell and early lineage markers using Taqman® low density array. No significant deviation in gene expression was observed between the two populations. Thus we established an efficient, complete xeno-free protocol forpropagation of human WJ-MSCs.Keywords: human serum, explant, trypLE, umbilical cord, FBS, bFGF
format article
author Venugopal P
Balasubramanian S
Sen Majumdar A
Ta M
author_facet Venugopal P
Balasubramanian S
Sen Majumdar A
Ta M
author_sort Venugopal P
title Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
title_short Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
title_full Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
title_fullStr Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
title_full_unstemmed Isolation, characterization, and gene expression analysis of Wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
title_sort isolation, characterization, and gene expression analysis of wharton’s jelly-derived mesenchymal stem cells under xeno-free culture conditions
publisher Dove Medical Press
publishDate 2011
url https://doaj.org/article/dc46bda55d9745d2bd2e4eb812b602ba
work_keys_str_mv AT venugopalp isolationcharacterizationandgeneexpressionanalysisofwhartonamprsquosjellyderivedmesenchymalstemcellsunderxenofreecultureconditions
AT balasubramanians isolationcharacterizationandgeneexpressionanalysisofwhartonamprsquosjellyderivedmesenchymalstemcellsunderxenofreecultureconditions
AT senmajumdara isolationcharacterizationandgeneexpressionanalysisofwhartonamprsquosjellyderivedmesenchymalstemcellsunderxenofreecultureconditions
AT tam isolationcharacterizationandgeneexpressionanalysisofwhartonamprsquosjellyderivedmesenchymalstemcellsunderxenofreecultureconditions
_version_ 1718403045301157888

Ejemplares similares