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pLT11 [LEU2 --> TRP1 converter]
pLT11 [LEU2 --> TRP1 converter]
規(guī)格:
貨期:
編號:B237349
品牌:Mingzhoubio

標準菌株
定量菌液
DNA
RNA

規(guī)格:
凍干粉
斜面
甘油
平板


產(chǎn)品名稱 pLT11 [LEU2 --> TRP1 converter]
商品貨號 B237349
Designations pLT11 [LEU2 --> TRP1 converter]
Depositors FR Cross
Biosafety Level 1
Vector Information
Size (kb): 10.5000000000000000
Vector: pLT11 (phagemid)
Construction: pBC KS+
Marker(s):TRP1,ampR,cmlR
Construct size (kb): 10.5
Features: gene disruption cassette: Leu2::TRP1/ampR
marker(s): cmlR
replicon: f1
replicon: pMB1
restriction site: BamHI, HpaI
restriction site: SalI, XhoI
Applications
YI-type (integrating) shuttle vector
host modification
marker swap vector LEU2 --> TRP1
Comments
Restriction digests of the clone give the following sizes (kb): BamHI--8.4, 2.1; BamHI/XhoI--4.9, 3.3, 2.2.
To convert the host phenotype from LEU2 to TRP1, transform with the XhoI+HpaI digested vector and select for Trp+ transformants.
Some combinations of marker swap plasmids and target locus may result in relatively high reversion rates. In most but not all cases the frequencies of successful convertants are greater than 30%.
A marker swap vector designed to change the S. cerevisiae host phenotype by one-step gene disruption of the LEU2 gene with the TRP1 and ampR markers.
When swapping markers on an episomal plasmid, appropriate phenotype may result from loss of the plasmid unless a second selectable or scorable marker is used to ensure plasmid maintenance.
Recommendation for verification: XhoI+HpaI--6.1, 4.4; BamHI+XhoI--5.1, 3.4, 2.0; BamHI--8.5, 2.0; HindIII+XhoI--6.3, 4.2.
Vector was constructed by replacing an internal EcoRI-EcoRV fragment of LEU2 with an XhoI-EcoRI fragment containing the TRP1 and ampR coding sequences.
Media ATCC Medium 1065 (see below) plus ampicillin (50 mcg/ml) plus chloramphenicol (20 mcg/ml) ATCC Medium 1065: Tryptone (Difco 0123), 10.0 g Yeast Extract (Difco 0127), 5.0 g NaCl, 10.0 g Distilled water, 1.0 L
Growth Conditions
Temperature: 37.0°C
References

Cross FR. 'Marker swap' plasmids: convenient tools for budding yeast molecular genetics. Yeast 13: 647-653, 1997. PubMed: 9200814

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