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pOT182
pOT182
規(guī)格:
貨期:
編號:B234564
品牌:Mingzhoubio

標(biāo)準(zhǔn)菌株
定量菌液
DNA
RNA

規(guī)格:
凍干粉
斜面
甘油
平板


產(chǎn)品名稱 pOT182
商品貨號 B234564
Designations pOT182
Depositors IL Lamont
Biosafety Level 1
Vector Information
Size (kb): 19.20
Vector: pOT182 (plasmid)
Construction: pSUP102::Tn5-B21, pBR325
Marker(s):ampR,cmlR,tetR,gtmR
Construct size (kb): 19.20
Features: insert detection: lacZ
marker(s): ampR, tetR, cmlR, gtmR
replicon: pMB1
Applications
integrating vector
promoter-cloning vector
Comments
Restriction digests of the clone give the following sizes (kb): EcoRI--13.0, 5.9; BamHI--12.0, 7.6; ClaI--17.0, 2.6; XhoI--19.6.
E. coli S17-1 contains an integrated derivative of RP4 and allows conjugative transfer of the vector.
Transconjugants are identified by resistance to tetracycline and carbenicillin.
In some strains, carbenicillin resistance may depend on transcription originating outside the transposon. This can provide a means for direct selection of recombinants in which the Tn has inserted downstream from an active promoter.
Chromosomal DNA fragments adjacent to the inserted lacZ gene can be cloned following digestion with HindIII, SalI, SmaI or XhoI and religation of the vector.
Fragments adjacent to the transposase can be cloned following digestion with BamHI, ClaI, EcoRI or SacI and religation.
It should also be possible to clone DNA flanking both sides of the transposon using BglII.
Religated vector can be transformed and propagated in any suitable E. coli, such as E. coli MC1061.
Integrating, "self-cloning" promoter probe vector. A mobilizable suicide plasmid that can be transferred to a broad range of Gram-negative bacteria.
The order of the major features in the plasmid is: IR - BamHI - lacZ(ClaI, SacI) - EcoRI - ampR - pMB1 ori - tetA - tetR(SalI, SmaI) - SmaI (2 sites) - tnp(HindIII, XhoI) - IR - BamHI - SalI - mob - cmlR(EcoRI) - ClaI - HindIII - gentamicinR.
Media ATCC® Medium 1946: Terrific broth (ATCC medium 1743) with 100 mcg/ml ampicillin
Growth Conditions
Temperature: 30.0°C
References

Merriman TR, Lamont IL. Construction and use of a self-cloning promoter probe vector for gram-negative bacteria. Gene 126: 17-23, 1993. PubMed: 8386128

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