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J. Biol. Chem., Vol. 255, Issue 24, 11957-11964, 12, 1980
EC Achberger and HR Whiteley
the ability of the core isolated from Escherichia coli RNA polymerase to
interact with specificity-determining subunits isolated from Bacillus
subtilis RNA polymerase has been determined by measuring the transcription
of "early" and "middle" genes of phage SP82. Two specificity-determining
subunits were tested: the sigma subunit and a 28,000 dalton (28 K) peptide
isolated from a modified polymerase produced at approximately 8 min after
infection of B. subtilis with SP82. Earlier experiments (Spiegelman, G. B.
and Whiteley, H. R. (1978) Biochem. Biophys. Res. Commun. 81, 1058-1065)
demonstrated that sigma and the 28K peptide are required for the
recognition of early and middle gene promoters, respectively, by the B.
subtilis core assembly. The present investigation showed that E. coli core
interacted more efficiently with the B. subtilis sigma than with the 28K
peptide, as judged by the rate of RNA synthesis. Early RNA was produced by
the E. coli and B. subtilis holoenzymes and by E. coli core supplenented
with B. subtilis sigma and only minor differences were found in comparisons
of transcripts by hybridization and by electrophoretic analysis.
Measurements of template specificity, the formation of stable enzyme . DNA
complexes, and the hybridization of transcripts to fragments of SP82 DNA
produced by digestion with restriction endonuclease Hha indicated that E.
coli core supplemented with the 28K-supplemented E. coli core with those
synthesized by the modified polymerase extracted from B. subtilis 8 min
after infection with SP82 suggest that both preparations recognized the
same initiation and termination sequences.
The interaction of Escherichia coli core RNA polymerase with specificity-determining subunits derived from unmodified and SP82- modified Bacillus subtilis RNA polymerase
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