Madhadron:ChromosomeMarker: Difference between revisions
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Two organisms already adapted thus: P1 phage, and pMT phage (from Y. pestis; uses a deletion of the the 23 N-terminal amino acids of ParB instead of the whole thing). | Two organisms already adapted thus: P1 phage, and pMT phage (from Y. pestis; uses a deletion of the the 23 N-terminal amino acids of ParB instead of the whole thing). | ||
The system depends on ihf genes in E. coli, and there is the HU homolog. | The system depends on ihf genes in E. coli, and there is the HU homolog. | ||
Alternately, make long strings of lexA sites. Mycobacterial LexA binds to Gram-positive style Cheo box. | |||
Gram negative SOS box: taCTGTatatananaCAGta | |||
Gram positive Cheo box: GAACNNNNGTTC | |||
Ligate 25 sites one after another, with lexA-YFP fusion? Use pMV361 as the carrier so as to get nice integration. | Ligate 25 sites one after another, with lexA-YFP fusion? Use pMV361 as the carrier so as to get nice integration. | ||
Check for Gram negative binding sequences in the smeg genome first. | Check for Gram negative binding sequences in the smeg genome first. |
Revision as of 11:10, 13 December 2006
This protocol is a port of the system described in Nielsen, Ottesen, etc. (2006) in Molecular Microbiology to mycobacteria.
Background
Two component system from phage: parS is a binding site for the ParB protein. parS is inserted in the chromosome (a single copy appears to be sufficient). ParB is expressed inducibly as a fusion protein with a GFP on a plasmid.
Two organisms already adapted thus: P1 phage, and pMT phage (from Y. pestis; uses a deletion of the the 23 N-terminal amino acids of ParB instead of the whole thing).
The system depends on ihf genes in E. coli, and there is the HU homolog.
Alternately, make long strings of lexA sites. Mycobacterial LexA binds to Gram-positive style Cheo box.
Gram negative SOS box: taCTGTatatananaCAGta
Gram positive Cheo box: GAACNNNNGTTC
Ligate 25 sites one after another, with lexA-YFP fusion? Use pMV361 as the carrier so as to get nice integration.
Check for Gram negative binding sequences in the smeg genome first.