Specific cleavage of bacteriophage R17 RNA by an endonuclease isolated from E. coli MRE-600.

1 March 1968

journal article
research article
Published by Proceedings of the National Academy of Sciences in Proceedings of the National Academy of Sciences

Vol. 59 (3) , 876-883
https://doi.org/10.1073/pnas.59.3.876

Abstract

A nuclease purified from a RNase I minus strain of Escherichia coli (MRE-600) specifically cleaves R17 RNA at a site about 1/3[image] of the way in the molecule from the 5[image]-end. The fragment that lacks the 5[image]-end of the original molecule is still able to direct the in-vitro synthesis of the phage RNA synthetase. The results suggest that this 2[beta] fragment has impaired ability to direct synthesis of coat protein. The 1[beta] fragment from the 5[image]-end of the RNA has relatively little template activity but directs synthesis of some coat protein-like material.

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