Dept
of Molecular Pharmacology |
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Retroviral cDNA and Peptide Libraries The power of complementation cloning, long appreciated in bacterial and yeast genetic systems, may now be more fully accessed for mammalian cells by applying retroviral delivery systems. The basic tenet of the approach is that using retroviruses large libraries of encoded objects (cDNAs, peptides, RNAs)-- among them desired objects capable of exerting a dominant phenotype on target cells-- can be transferred to target mammalian cells. By applying appropriate genetic selections one can isolate those cells expressing the object of interest from among a background of unwanted objects. We have applied this in two main areas:
Other applications of libraries include:Mutant cDNA libraries in which PCR or other mutagenesis is used to mutate a known cDNA and a library selection system is set to find those mutant cDNAs that survive the selection. This can be used to find, in a non-biased and interesting manner, new sites on proteins that are not readily found using standard mutagenic approaches. cDNA fragment libraries. Pioneered by Igor Roninson at the University of Chicago this approach uses randomly fragmented cDNA expressed in retroviral backbones. The approach allows for "mini-domain" interference in signaling systems with the notion that the fragments' ability to interfere, and its constitution, allows for biological inferences to be made. Ribozyme Libraries. A variety of ribozymes have been encoded in retroviruses. Some individuals have suggested that by randomizing the targeting sequence, and setting appropriate selection criteria, one can isolate ribozymes with specific properties that are capable of cleaving "unknown" mRNAs. Of course, the inference is that once the ribozyme is sequenced one will be able to soon discover the nature of the target RNA and then determine how the cleavage event determines the selected event. |
Related links:
Also of interest is the PNAS manuscript on which this cDNA library work was based by Kitamura T, et al.
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