Animal models are essential for studying basic biological processes, elucidating the root causes of disease, and developing treatment regimens for disease. The mouse has proven to be particularly amenable to genetic manipulation, allowing researchers to design mouse models specific for their work. A great number of useful mouse models have been generated by inserting various genes into mice (gain of function), or disrupting/deleting various genes from the mouse genome (loss of function). However, there exist no rapid, simple techniques to introduce a precise mutation at a particular spot in the mouse genome (correction of function or change of function). The current standard technology is extremely cumbersome and always involves concomitant insertions or alterations in addition to the desired point mutation. We are therefore attempting to adapt technologies being developed in the gene therapy field for effecting somatic cell gene repair, to induce specific point mutations into the mouse genome.? ? Our general protocol involves microinjecting of modified single stranded DNA (ssDNA), alone or in combination with other factors, into pronuclei of one celled mouse embryos. Manipulated embryos are incubated up to the blastula stage, at which point they are examined for presence of the desired mutation. In this way, we are searching for factors that could increase the frequency of targeted DNA point mutations, and developing an understanding of the mechanisms controlling this type of gene alteration. While working to produce an efficient high throughput assay, we have been using PCR-based restriction fragment length polymorphism (RFLP) assay to detect point mutation introduced into genomic DNA. Several experiments, reported previously, have yielded promising results. Our results are consistent with mounting evidence in the literature that gene editing by this mechanism involves components of the homologous recombination pathway, which have been shown to be present in mouse ova and preimplantation stage embryos, and suggest an inhibitory role for the non-homologous end-joining pathway, which is generally the preferential mode of DNA repair in mammalian cells.? ? The RFLP-based technique is extremely time consuming, and, for low DNA copy number, could result in questionable fidelity. To improve the detection method, we are developing transgenic mouse lines in which correction of a mutation in a fluorescent protein will give an instant read-out, and many embryos can be screened simultaneously. We previously engineered a cassette encoding a bicistronic mRNA (mutated red fluorescent protein [DsRed] / an IRES element / green fluorescent protein). All mouse embryos expressing the transgene should fluoresce green (endogenous control for transgene expression), but only embryos in which the point mutation in DsRed has been corrected should also fluoresce red. We have used several enhancer/promoter elements, which have been used successfully in preimplantation stage mouse embryos or mouse ES cells, to drive expression of the cassette. ? ? A successful promoter would induce easily detectable levels of fluorescent protein expression at the earliest stages of embryo development. All promoter/fluorescent protein transgenes were constructed and tested for expression of EGFP and DsRed in both transient assays in mouse embryos and in F1 transgenic mouse embryos. Expression of green or red proteins from the mPGK promoter was detected neither in transient assays nor in transgenic mouse embryos. The mPGK promoter with adenovirus tripartite leader enhancer construct was able to induce expression of EGFP, but not DsRed, in transient assays, and a transgenic mouse line failed to express any detectable fluorescent protein. The hCMV IE promoter / enhancer, the hCMV IE enhancer / chicken betta-actin promoter and partial intron / rabbit betta-globin partial intron, and the EF1alpha promoter all induce detectable EGFP and DsRed expression in mouse embryos during transient assays. For the last two constructs, expression was extremely high. However, transgenic mice with the hCMV IE promoter / enhancer construct expressed EGFP only after embryo hatching, and did not express DsRed. The construct carrying the chicken beta-actin promoter with the hCMV IE enhancer produces detectable expression of both fluorescent proteins in transgenic mouse embryos. EGEP was visible at the early blastula stage, and DsRed fluorescence appeared at the late blastula stage. These data imply that expression of DsRed protein is not lethal for mouse embryos, which has been suggested in the literature. Surprisingly, the EF1alpha promoter construct, with mutated DsRed protein, was able to generate green fluorescent protein in eight cell stage embryos. A line of transgenic mice with the EF1alpha promoter / mutated red fluorescent protein / an IRES element / green fluorescent protein construct appears to be extremely promising at this time. Establishment and characterization of this transgenic mouse line is ongoing.

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Intramural Research (Z01)
Project #
1Z01EY000371-06
Application #
7322357
Study Section
(TAGM)
Project Start
Project End
Budget Start
Budget End
Support Year
6
Fiscal Year
2006
Total Cost
Indirect Cost
Name
U.S. National Eye Institute
Department
Type
DUNS #
City
State
Country
United States
Zip Code