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Publication : Expression of laminin chains by central neurons: analysis with gene and protein trapping techniques.

First Author  Yin Y Year  2003
Journal  Genesis Volume  36
Issue  2 Pages  114-27
PubMed ID  12820173 Mgi Jnum  J:85792
Mgi Id  MGI:2676922 Doi  10.1002/gene.10206
Citation  Yin Y, et al. (2003) Expression of laminin chains by central neurons: analysis with gene and protein trapping techniques. Genesis 36(2):114-27
abstractText  Laminins exert numerous effects on neurons in vitro, but expression of laminin subunit genes by neurons in vivo remains controversial. To reexamine this issue, we generated mice from ES cells in which the laminin alpha1, alpha5, beta1, and gamma1 genes had been 'trapped' by insertion of a histochemically detectable selectable marker, betageo (beta-galactosidase fused to neomycin phosphotransferase). The presence of laminin-betageo fusion proteins was assayed histochemically and immunochemically, revealing expression of laminin beta1 and gamma1 genes, but not alpha chain genes, by defined subsets of neurons in brain and retina. We also used the gene traps in a novel way to assay expression of endogenous laminin subunits, which were barely detectable by ordinary immunohistochemical methods. The trapping vector included a transmembrane domain that anchors proteins otherwise destined for secretion. Laminin alpha/beta/gamma heterotrimers are assembled intracellularly, and we show that the trapped laminin gamma1 fusion protein 'co-trapped' endogenous beta1 intracellularly. The laminin gamma1 fusion was also able to co-trap transgene-derived alpha chains, but we detected no co-trapped endogenous alpha chains. The co-trapping method may be generally useful for identifying proteins or isolating protein complexes associated with trapped gene products.
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