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Journal home Advance online publication Current issue Archive Press releases Free Association (blog) Supplements Focuses Guide to authors Online submission For referees Free online issue Contact the journal Subscribe Advertising work@npg Reprints and permissions About this site For librarians   NPG Resources Nature Nature Biotechnology Nature Cell Biology Nature Medicine Nature Methods Nature Reviews Cancer Nature Reviews Genetics Nature Reviews Molecular Cell Biology news@nature.com Nature Conferences Nature Reports Stem Cells RNAi Gateway NPG Subject areas Biotechnology Cancer Chemistry Clinical Medicine Dentistry Development Drug Discovery Earth Sciences Evolution & Ecology Genetics Immunology Materials Science Medical Research Microbiology Molecular Cell Biology Neuroscience Pharmacology Physics Browse all publications Technical Report Nature Genetics  36, 190 - 196 (2004) Published online: 4 January 2004; | doi:10.1038/ng1290 Enzymatic production of RNAi libraries from cDNAs Daisuke Shirane1, 2, Kohtaroh Sugao1, 2, Shigeyuki Namiki1, Mao Tanabe1, Masamitsu Iino1 & Kenzo Hirose1 1  Department of Pharmacology, Graduate School of Medicine, The University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan. 2  These authors contributed equally to this work. Correspondence should be addressed to Kenzo Hirose kenzo@m.u-tokyo.ac.jpRNA interference (RNAi) induced by small interfering (siRNA) or short hairpin RNA (shRNA) is an important research approach in mammalian genetics. Here we describe a technology called enzymatic production of RNAi library (EPRIL) by which cDNAs are converted by a sequence of enzymatic treatments into an RNAi library consisting of a vast array of different shRNA expression constructs. We applied EPRIL to a single cDNA source and prepared an RNAi library consisting of shRNA constructs with various RNAi efficiencies. High-throughput screening allowed us to rapidly identify the best shRNA constructs from the library. We also describe a new selection scheme using the thymidine kinase gene for obtaining efficient shRNA constructs. Furthermore, we show that EPRIL can be applied to constructing an RNAi library from a cDNA library, providing a basis for future whole-genome phenotypic screening of genes. MORE ARTICLES LIKE THIS These links to content published by NPG are automatically generated. NEWS AND VIEWS RNA interference Human genes hit the big screen Nature News and Views (25 Mar 2004) Dicing with siRNA Nature Biotechnology News and Views (01 Feb 2005) RESEARCH Circumventing tolerance to a human MDM2-derived tumor antigen by TCR gene transfer Nature Immunology Article (01 Oct 2001) See all 40 matches for Research  Top Abstract Previous | Next Table of contents Full text Download PDF Send to a friend Open Innovation Challenges Efficient Chromosome Doubling: Plant Cell Division Deadline: Jul 15 2009 Reward: $20,000 USD The Seeker is looking for an efficient chromosome doubling method in plants and in particular, metho... Fast Growth of Transformed Soybean Shoots Deadline: Jul 15 2009 Reward: $10,000 USD A method for accelerating growth of soybean shoots is desired. More Challenges Powered by: nature jobs Professorship in Functional Genomics of Fungi University of Natural Resources and Applied Life Sciences Vienna Vienna 1190 Austria Postdoctoral Research Fellow ? Andy Chan?s Lab / Immunology Genentech South San Francisco, CA, USA More science jobs Post a job for free Figures & Tables Supplementary info Export citation Search buyers guide:   ADVERTISEMENT

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