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65 research outputs found

Articular cartilage proteoglycan biosynthesis and sulfation (Nivelruston proteoglykaanien biosynteesi ja sulfaatio)

Author: Qu Chengjuan
Publication venue: University of Kuopio
Publication date
Field of study

UEF Electronic Publications

The Effects of Chondroitin and/or Glucosamine on Patients with Kashin-Beck Disease

Author: Chengjuan Qu
Danyang Li
Fangfang Yu
Jianhua Yi
Jing Han
null null
null null
null null
Xiaofang Wu
Xiong Guo
Zuyong Wang
Publication venue: Bonoi Science Advancement and Education LLC
Publication date: 20/02/2016
Field of study

Crossref

Scaffold-free approach produces neocartilage tissue of similar quality as the use of HyStem™ and Hydromatrix™ scaffolds

Author: AJ Hayes
B Bosnakovski
C Qu
Chengjuan Qu
CJ Qu
CR Correia
D Stoppoloni
E Tchetina
EB Hunziker
EB Hunziker
G Tani
GA Gilpin
GD DuRaine
GJ Osch van
HS Yoo
IE Erickson
J Huang
Janne H. Ylärinne
JC Hu
JH Ylärinne
K Park
KA Athanasiou
KS Furukawa
KW Ng
L Donaldson
L Galois
M Sato
MD Buschmann
Mikko J. Lammi
R Holmdahl
RH Harrison
RW Farndale
T Miyazaki
T Nagai
TE Hardingham
V Lefebvre
Y Mori
YC Cheuk
Publication venue: 'Springer Science and Business Media LLC'
Publication date
Field of study

Crossref

Nivelruston proteoglykaanien biosynteesi ja sulfaatio

Author: Qu Chengjuan
Publication venue: Kuopio
Publication date: 02/11/2007
Field of study

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UEF eRepository

Faculty Opinions recommendation of Nasal chondrocyte-based engineered autologous cartilage tissue for repair of articular cartilage defects: an observational first-in-human trial.

Author: Chengjuan Qu
Mikko Lammi
Publication venue: Faculty Opinions Ltd
Publication date: 17/08/2017
Field of study

Crossref

Chondrocyte-specific gene expressions in human embryonic stem cells differentiated under feeder-free culture conditions

Author: Lammi Mikko,
Qu Chengjuan,
Publication venue
Publication date: 01/01/2017
Field of study

Background: Chondrogenic differentiation of human embryonic stem cells (hESCs) has been investigated by maintenance of 3-dimensional cultures in the presence of various exogenous growth factors added during defined stages of culture, or in cocultures with primary chondrocytes, which makes the cultivation process rather complex. Thus, there is a need for easier and more handy expansion and differentiation protocols.Objective: The present study is aimed to investigate the potential of hESCs for chondrogenic differentiation in simpler culture conditions.Methods: The hESCs were directly cultured for 3 weeks on feeder-free gelatin-coated plates in chondrocyte culture medium without any growth factor supplements after 6-day culture on feeder-free gelatin-coated plate with conditioned medium.Results: Immunocytochemical and gene expression analyses indicated that these human directly differentiated cells (hDDCs), which derived from the hESCs, abundantly expressed Sox9, aggrecan, and procollagen a1(II) mRNAs. Upon further passaging, the hDDCs behaved similarly to primary chondrocytes, although the aggrecan mRNA expressions were maintained at a relatively constant level throughout passaging. The procollagen a1(II) mRNAs expression was high in the beginning of the hDDC culture, but declined upon further passaging, which is typical for the primary chondrocytes. The hDDCs could be easily expanded in the monolayer culture using chondrocyte culture medium. Differentiation assays showed that the hDDCs could be differentiated towards chondrocytes, but not adipocytes or osteoblasts.Conclusion: Our data suggests that the chondrogenic gene expression could be induced in the directly differentiated hESCs without a need for chondrocyte coculture. In contrast, no osteogenic or adipogenic differentiation was observed.</p

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