Price Information
| Cat No. | Plasmid Name | Availability | Add to cart |
|---|---|---|---|
| V014951 | pLV-7×SMAD-Fluc-Puro | In stock, 1 week for quality controls |
Buy one, get one free! |
Two tubes of lyophilized plasmid will be delivered, each tube is about 5µg.
Basic Vector Information
- Vector Name:
- pLV-7×SMAD-Fluc-Puro
- Antibiotic Resistance:
- Ampicillin
- Length:
- 8143 bp
- Replication origin:
- ori
pLV-7×SMAD-Fluc-Puro vector Map
Plasmid Protocol
1. Centrifuge at 5,000×g for 5 min.
2. Carefully open the tube and add 20 μl of sterile water to dissolve the DNA.
3. Close the tube and incubate for 10 minutes at room temperature.
4. Briefly vortex the tube and then do a quick spin to concentrate the liquid at the bottom. Speed is less than 5000×g.
5. Store the plasmid at -20 ℃.
6. The concentration of plasmid re-measurement sometimes differs from the nominal value, which may be due to the position of the lyophilized plasmid in the tube, the efficiency of the re-dissolution, the measurement bias, and adsorption on the wall of the tube, therefore, it is recommended to transform and extract the plasmid before using it
General Plasmid Transform Protocol
1. Take one 100μl of the competent cells and thaw it on ice for 10min, add 2μl of plasmid, then ice bath for 30min, then heat-shock it at 42℃ for 60s, do not stir, and then ice bath for 2min.
2. Add 900μl of LB liquid medium without antibiotics, and incubate at 37℃ for 45min (30℃ for 1-1.5 hours) with 180rpm shaking.
3. Centrifuge at 6000rpm for 5min, leave only 100μl of supernatant to resuspend the bacterial precipitate and spread it onto the target plasmid-resistant LB plate.
4. Invert the plate and incubate at 37℃ for 14h, or at 30℃ for 20h.
5. Pick a single colony into LB liquid medium, add the corresponding antibiotics, incubate at 220rpm for 14h, and extract the plasmid according to the experimental needs and the instructions of the plasmid extraction kit.
pLV-7×SMAD-Fluc-Puro vector Sequence
LOCUS Exported 8143 bp DNA circular SYN 14-JUN-2024
DEFINITION Exported.
ACCESSION V014951
VERSION .
KEYWORDS .
SOURCE synthetic DNA construct
ORGANISM synthetic DNA construct
REFERENCE 1 (bases 1 to 8143)
TITLE Direct Submission
REFERENCE 2 (bases 1 to 8143)
AUTHORS .
TITLE Direct Submission
COMMENT SGRef: number: 1; type: "Journal Article"
FEATURES Location/Qualifiers
source 1..8143
/mol_type="other DNA"
/organism="synthetic DNA construct"
LTR 117..750
/label=3' LTR
/note="3' long terminal repeat (LTR) from HIV-1"
misc_feature 797..922
/label=HIV-1 Psi
/note="packaging signal of human immunodeficiency virus
type 1"
misc_feature 1415..1648
/label=RRE
/note="The Rev response element (RRE) of HIV-1 allows for
Rev-dependent mRNA export from the nucleus to the
cytoplasm."
CDS 1833..1877
/label=gp41 peptide
/note="antigenic peptide corresponding to amino acids 655
to 669 of the HIV envelope protein gp41 (Lutje Hulsik et
al., 2013)"
CDS 2026..2067
/label=Protein Tat
/note="Protein Tat from Human immunodeficiency virus type 1
group M subtype B (isolate WMJ22). Accession#: P12509"
misc_feature 2164..2281
/label=cPPT/CTS
/note="central polypurine tract and central termination
sequence of HIV-1"
protein_bind join(2297..2304,2309..2316,2327..2334,2341..2348,2356..2363,
2371..2378,2385..2392)
/label=7xSMAD
/bound_moiety="SMAD binding motif 7 copies"
promoter 2445..2476
/label=minP
/note="minimal TATA-box promoter with low basal activity"
CDS 2555..4204
/label=luciferase
/note="firefly luciferase"
misc_feature 4259..4845
/label=IRES2
/note="internal ribosome entry site (IRES) of the
encephalomyocarditis virus (EMCV)"
CDS 4865..5461
/label=PuroR
/note="puromycin N-acetyltransferase"
LTR 5667..5900
/label=3' LTR (Delta-U3)
/note="self-inactivating 3' long terminal repeat (LTR) from
HIV-1"
polyA_signal 6057..6281
/label=bGH poly(A) signal
/note="bovine growth hormone polyadenylation signal"
promoter 6377..6481
/label=AmpR promoter
CDS 6482..7339
/label=AmpR
/note="beta-lactamase"
rep_origin 7513..8101
/direction=RIGHT
/label=ori
/note="high-copy-number ColE1/pMB1/pBR322/pUC origin of
replication"