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JBC, Vol. 250, Issue 8, 3050-3056, Apr, 1975
H. D. Robertson and J. J. Dunn
We have studied the nuclease activities present in preparations of
Escherichia coli RNase III and the "sizing factor" responsible for specific
processing of several RNA species. RNase III preparations contain three
activities: one which solubilizes stable RNA:RNA duplexes; one which
solubilizes the RNA of DNA:RNA hybrids; and one which processes the
polycistronic mRNA of bacteriophage T7 in a manner identical with sizing
factor. We show that the activity against the RNA of DNA:RNA hybrids can
be removed, but that the activity which cleaves RNA:RNA duplexes and that
responsible for specific processing of phage T7 polycistronic mRNA appear
to be identical by several biochemical criteria. In addition, partially
purified enzyme fractions from mutants lacking these two activities contain
substantial amounts of activity against the RNA of DNA:RNA hybrids. We have
also defined several properties of the two activities solubilize RNA:RNA
duplexes and RNA of DNA:RNA hybrids. Average oligonucleotide chain length
in an exhaustive digest of double-stranded RNA is about 15 bases, while
that in a digest of the RNA in DNA:RNA hybrids is less than 10 bases.
Direct analysis shows that both activities cleave RNA chains to yield
5'-phosphate and 3'-hydroxyl termini. All four bases can reside at the 5'
end of the resulting oligonucleotides, although both activities show a mild
preference for certain bases. These results and previous findings allow us
to specify the probably size and structure of potential cleavage sites for
these enzymes in biological RNA molecules.
Ribonucleic acid processing activity of Escherichia coli ribonuclease III
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N. Beguiristain, H. D. Robertson, and J. Gomez RNase III cleavage demonstrates a long range RNA: RNA duplex element flanking the hepatitis C virus internal ribosome entry site Nucleic Acids Res., September 16, 2005; 33(16): 5250 - 5261. [Abstract] [Full Text] [PDF] |
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