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Library Resource Designed to Uncover the Role of microRNAs

By LabMedica International staff writers
Posted on 17 Aug 2011
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The first mammalian microRNA knockout resource--mirKO--will soon be released.

The research toolbox of mutant mouse embryonic stem (ES) cells, in which individual or clustered groups of microRNA genes have been deleted, will help researchers clarify the role of microRNAs in health and disease. Utilizing these tools researchers can create cells or mice lacking specific microRNAs, study expression using fluorescent markers, or inactivate the gene in specific tissues or at specific times in development.

A new resource to define the roles of microRNAs was described August 7, 2011, in the journal Nature Biotechnology. The resource, mirKO, gives researchers access to tools to study the biologic role and significance for human health of these genes. This is the first mammalian microRNA knockout resource, or library; the only other comprehensive resource of mutated microRNA genes is that for the nematode worm.

microRNAs--first named only 10 years ago--are encoded by more than 500 genes that are forecast to regulate about one third of protein-coding genes. Consisting of short stretches of 21 to 23 nucleotides, microRNAs act by interfering with the activity of messenger RNAs. Studies over the past five years have shown that microRNAs are likely to play significant roles in disease such as cancer and disorders of the heart, the immune system, and auditory systems.

“We have generated a resource of microRNA knockout alleles in mouse ES cells that are standardized with respect to design and genetic background that researchers can access through repositories,” said Dr. Haydn Prosser, lead author on the research from the Wellcome Trust Sanger Institute (Hoxton, UK). “In many cases, microRNAs with overlapping messenger RNA target specificities occur at multiple locations throughout the genome. To address these complexities a comprehensive resource is valuable to enable the creation of compound mutants in cells or mice.”

The first phase of the research was to develop DNA vectors to target the microRNA genes: the team produced two alternative vectors that could, if desired, be used to knock out both copies of a particular microRNA in mouse ES cells.

The investigators inserted newly designed DNA vectors in place of the microRNA genes, successfully knocking out approximately 400 up to now. “The biology of microRNAs will be revealed only when we can rigorously examine their activity, their role in individual tissues, and at specific times in development,” remarked Prof. Allan Bradley, senior author on the study and director emeritus of the Sanger Institute. “Our paper shows that the tools within mirKO can do that. We have tagged genes with a color reporter, developed a mutation that can be induced when required and produced mice carrying mutations. This is an important proof of principle.”

In earlier research, Prof. Bradley’s team demonstrated that a specific microRNA played a role in the development of a component of the immune system: in its absence, mice develop symptoms similar to those of human autoimmune disease and are less resistant to infection.

The resource is built on cassettes of genetic components that can be swapped through a technology called recombinase mediated cassette exchange (RMCE). “We have designed the targeted alleles to be adaptable in order that researchers can efficiently alter particular microRNA loci in a multitude of alternative ways to provide information additional to straightforward null mutants. In this respect we have developed a research toolbox that will help researchers define the role of microRNAs in health and disease,” said Dr. Prosser.

In one configuration, the wild-type microRNA locus was reconstituted while being flanked by recombinase sites in order to facilitate time--or tissue-specific expression. A second RMCE cassette contains a gene that generated a red fluorescent protein: when this is converted into a mutated microRNA gene, it reflects the activity of the mouse microRNA gene so its activity can be examined. The team showed that this method accurately reflected the known activity of two microRNA loci.

The developing suite of tools has already been invaluable to researchers. “This is clearly a valuable resource which will make research easier and more efficient,” stated Eric Miska, a group leader at the Wellcome Trust/Cancer Research UK Gurdon Institute (Cambridge, UK). “In our research into regulatory RNAs, we are using this resource to investigate the role of individual microRNAs during early development and how their deregulation might contribute to the etiology of cancer.”

Related Links:

Wellcome Trust Sanger Institute


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