Dlx5 regulation of mouse osteoblast differentiation mediated by avian retrovirus vector

Dlx5 regulation of mouse osteoblast differentiation mediated by avian retrovirus vector

To study the effect of Dlx5 introduced by replication-competent avian splice-acceptor (RCAS) in mouse calvarial and bone marrow stromal cells, and to demonstrate that RCAS vector can be a useful system for studying gene expression in mammalian cells derived from Beta-AKE mouse. Beta-AKE mouse used i...

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Published in:Croatian medical journal Vol. 44; no. 4; pp. 407 - 411
Main Authors: Erceg, Ivana, Tadić, Tade, Kronenberg, Mark S, Marijanović, Inga, Lichtler, Alexander C
Format: Journal Article
Language:English
Published: Croatia 01-08-2003
Subjects:
Animals
Blotting, Northern
Bone Marrow Cells - physiology
Cell Differentiation - genetics
Cells, Cultured
Gene Expression Regulation, Developmental
Genetic Vectors
Homeodomain Proteins - genetics
In Situ Hybridization
Mice
Mice, Transgenic
Osteoblasts - physiology
Retroviridae - genetics
RNA, Messenger - analysis
Sensitivity and Specificity
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Summary:To study the effect of Dlx5 introduced by replication-competent avian splice-acceptor (RCAS) in mouse calvarial and bone marrow stromal cells, and to demonstrate that RCAS vector can be a useful system for studying gene expression in mammalian cells derived from Beta-AKE mouse. Beta-AKE mouse used in experiments is a transgenic mouse line expressing the receptor for the Bryant polymerase subgroup A of RCAS vector (RCAS-BP(A) vector). Primary calvarial osteoblast cultures were obtained from 7-day-old Beta-AKE mice. Bone marrow stromal cells were derived from the long bones of 8-week-old Beta-AKE mice. Expression of genes cloned into RCAS vector in mouse cells was first established by detecting green fluorescent protein (GFP) in cells infected with RCAS-BP(A)-GFP sapphire by using fluorescence microscopy. Cells were then infected with RCAS-BP(A)-Dlx5 or RCAS-BP(A) alone as a control, for three days. After differentiation, cells were harvested for mRNA analysis at different time points (day 6 or 7, 11 or 12, 14 or 18, and 21 or 25). The cells were cultured in the presence of ascorbic acid and Beta-glycerophosphate, which promotes osteoblastic differentiation. Mouse calvarial and bone marrow stromal cells infected with RCAS-BP(A)-GFP sapphire were fluorescent compared with the controls. Both types of cells infected with RCAS-BP(A)Dlx5 consistently expressed increased levels of bone differentiation markers - type 1 collagen (Col1a1), osteocalcin, and bone sialoprotein mRNA. RCAS-BP(A) vector transduction of cells from Beta-AKE mice is a useful system for studying the role of gene expression in mouse osteoblastic cells. Dlx5 overexpression mediated by an RCAS-BP(A) vector stimulates mouse osteoblastic differentiation in Beta-AKE transgenic mice. Dlx5 induces osteoblast differentiation from bones formed either by endochondral or by membranous ossification.
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ISSN:0353-9504