| Literature DB >> 19279730 |
Wen-Chin Lee1, Rachel Berry, Peter Hohenstein, Jamie Davies.
Abstract
Removing the function of a specific gene from a developing organ, by making a 'knockout' mouse, is a powerful method for analyzing the molecular pathways that control organogenesis. The technique is expensive, though, in terms of time and money, and complex strategies for producing conditional knockouts are needed for genes that are essential for early development of the embryo, for which an unconditional knockout would be lethal before the organ of interest begins to form. Small interfering RNAs (siRNAs) offer a method of knocking down the expression of specific genes with no need for genomic manipulation. Almost as soon as they had been discovered, siRNAs began to be used to explore the molecular biology of mammalian cells in conventional, two-dimensional culture. They have now also been applied successfully, by several groups, to knock down specific genes in various organ rudiments developing in organ culture. This article reviews the basic technique of siRNA-mediated gene knockdown and how it is being applied to organ culture. It also reviews some of the current problems and challenges in the field, and the ways in which these problems are likely to be overcome.Entities:
Keywords: 3D culture; RNAi; organ culture; organ development; organogenesis; siRNA
Year: 2008 PMID: 19279730 PMCID: PMC2634977 DOI: 10.4161/org.4.3.6642
Source DB: PubMed Journal: Organogenesis ISSN: 1547-6278 Impact factor: 2.500