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Mol Cell Biol, June 1998, p. 3455-3465, Vol. 18, No. 6
Department of Biology, University of
Rochester, Rochester, New York 14627
Received 8 January 1998/Returned for modification 20 February
1998/Accepted 18 March 1998
R2 is a non-long terminal repeat retrotransposable element that
inserts itself site specifically in the 28S rRNA genes of arthropods.
The 120-kDa protein encoded by R2 has been shown to cleave one strand
of the 28S gene at the target site and to use the 3' hydroxyl group
generated from this nick to prime reverse transcription of its own RNA.
This reaction has been termed target-primed reverse transcription
(TPRT). Cleavage of the second DNA strand can occur in the presence or
absence of reverse transcription but requires RNA. In this study, more
sensitive in vitro assays have enabled further characterization of
these reactions. R2 protein is capable of only a single round of TPRT
because, once bound to the target DNA, it does not dissociate at
physiological ionic strengths. Analysis of the role of RNA in the DNA
cleavage reaction has revealed that the binding of RNA induces the R2
protein to form a multimeric complex. While larger complexes may form,
the active component appears to be a dimer based on sedimentation studies and the change in stoichiometry of the cleavage reaction from a
1:1 ratio of protein subunit to target DNA in the absence of RNA to a
2:1 ratio of subunit to DNA target in the presence of RNA. Nonspecific
RNA can also induce formation of this RNA-protein (RNP) complex, but
the association of the protein with R2 RNA is stronger as revealed by
its stability in 0.4 M NaCl. Finally, formation of the RNP complex
gives rise to a 150-fold increase in the ability of the R2 endonuclease
to find the target site. The specificity of this RNP complex is
sufficiently great that it can find the 28S gene target site and
conduct the TPRT reaction with total genomic DNA.
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
RNA-Induced Changes in the Activity of the
Endonuclease Encoded by the R2 Retrotransposable Element
*
Corresponding author. Mailing address: Department of
Biology, University of Rochester, Rochester, NY 14627. Phone: (716)
275-7274. Fax: (716) 275-2070. E-mail:
eick{at}uhura.cc.rochester.edu.
Mol Cell Biol, June 1998, p. 3455-3465, Vol. 18, No. 6
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
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