Difference between revisions of "PMID:14430363"
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== Materials and Methods Used == | == Materials and Methods Used == | ||
− | + | *Strains: | |
+ | **Hfr (''z<sup>+</sup>i<sup>+</sup>) | ||
+ | **F<sup>-</sup> (z<sup>-</sup>i<sup>-</sup>) | ||
+ | |||
+ | *Conjugation | ||
+ | |||
+ | *Reagents | ||
+ | **Streptomycin | ||
+ | **Chloramphenicol | ||
+ | **5-methytryptophan | ||
+ | **Duponol C(Na lauryl sulfate) | ||
==Phenotype Annotations== | ==Phenotype Annotations== |
Revision as of 17:29, 22 November 2010
Citation |
PARDEE, AB and PRESTIDGE, LS (1959) On the nature of the repressor of beta-galactosidase synthesis in Escherichia coli.Biochim. Biophys. Acta 36:545-7 |
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Abstract |
No abstract in PubMed |
Links | |
Keywords |
Escherichia coli; Glycoside Hydrolases |
edit table |
Main Points of the Paper
- Hfr(z+i+) X F-(z-i-):
- within a few minutes of the time of entry of the z+i+ genes (which are closely linked) the synthesis of β-galactosidase commenced at maximal velocity in the absence of extracellular inducer
- inducible i+ allele appears dominant over the constitutive i- allele
- The idea that i+ could control the synthesis of a destructive enzyme which removes an endogenous intracellular inducer was eliminated due to observation from this paper (Figure 1, curves C & D).
- The presence of 5-methyltryptophan enhances mating efficiency
- The data in this paper may suggest that:
- an inducer-destroying enzyme is not responsible for the difference between inducibility and constitutivity
- the repressor is not a protein, although the authors state this conclusion is open to doubt (evidence to refute this conclusion is shown here).
Materials and Methods Used
- Strains:
- Hfr (z+i+)
- F- (z-i-)
- Conjugation
- Reagents
- Streptomycin
- Chloramphenicol
- 5-methytryptophan
- Duponol C(Na lauryl sulfate)
Phenotype Annotations
<protect>
Species | Taxon ID | Strain | Gene (if known) | OMP | Phenotype | Details | Evidence | Notes |
---|---|---|---|---|---|---|---|---|
edit table |
</protect>