Abstract
The E. coli rnc gene encodes the double-stranded, RNA-specific ribonuclease III (RNaseIII). A novel bacteriophage, gy1, was isolated, and its propagation in E. coli was shown to depend on the expression of RNaseIII in the cell. (a) gyl has a low efficiency of plating on rnc+ strains and a high efficiency of plating on a rnc-E. coli strain harboring the rnc 105 point mutation that renders its RNaseIII product inactive. (b) gy1 has a high efficiency of plating on rnc- strains in which the rnc gene is disrupted by a ΔTn10 insertion. (c) Plasmids harboring a rnc+ gene that were introduced into the rnc- strains described above reduced the efficiency of plating of gy1.
| Original language | English |
|---|---|
| Pages (from-to) | 63-66 |
| Number of pages | 4 |
| Journal | Current Microbiology |
| Volume | 24 |
| Issue number | 2 |
| DOIs | |
| State | Published - Feb 1992 |
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