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New yeast/E. coli/Drosophila triple shuttle vectors for efficient generation of Drosophila P element transformation constructs |
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| Authors: | Achim Paululat Jürgen J Heinisch |
| Institution: | 1. University of Osnabrück, Faculty of Biology, Department of Zoology and Developmental Biology, Barbarastr. 11, D-49076 Osnabrück, Germany;2. University of Osnabrück, Faculty of Biology, Department of Genetics, Barbarastr. 11, D-49076 Osnabrück, Germany |
| Abstract: | We have generated a set of novel triple shuttle vectors that facilitate the construction of Drosophila-P-element transformations vectors. These YED-vectors allow the insertion of any kind of sequence at any chosen position due to the presence of a yeast casette which ensures replication and allows for homologous recombination in Saccharomyces cerevisiae. As a proof of principle we generated several reporter constructs and tested them in transgenic flies for expression and correct subcellular localization. YED-vectors can be used for many purposes including promoter analysis or the expression of tagged or truncated proteins. Thus, time-consuming conventional restriction site based multi-step cloning procedures can be circumvented by using the new YED-vectors. The new set of triple shuttle vectors will be highly beneficial for the rapid construction of complex Drosophila transformation plasmids. |
| Keywords: | GFP Green Fluorescence Protein PCR polymerase chain reaction nGFP nuclear GFP cytGFP cytoplasmic GFP NLS Nuclear Localization Sequence YED Yeast&ndash E coli&ndash Drosophila |
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