Addgene - pLVPT-rtTR-KRAB-2SM2 Plasmid Data

Gene/insert name:		mPGK, GFP, rtTR-KRAB-2SM2, Tet-off
Insert size (bp):		Unknown
Vector backbone:		None (Search Vector Database)
Type of vector:		Mammalian expression,Lentiviral
Backbone size (bp):		11645
5' Sequencing primer:		See map (List of Sequencing Primers)
Bacteria resistance:		Ampicillin
High or low copy:		High Copy
Grow in standard E. coli @ 37C:		No
Please specify bacterial strain for growth and growth condition:		Use Stbl3 or HB101 to reduce chance of recombination. Grow at 37C
Sequence:		View sequence
Author's Map:		View map
Plasmid Provided In:		Stbl3
Principal Investigator:		Patrick Aebischer
Terms and Licenses:		MTA, Tet Systems LULL

Comments: Transgenes can be expressed from any RNA Pol II promoter as part of bicistronic unit comprising the KRAB-based repressor; tetO sequences are inserted into the vector LTR. Tet-on and Tet-off versions rely on repressors that bind in the absence or the presence of doxycycline, respectively. Addition of Pol III promoter-small hairpin RNA cassette allows for drug-controllable RNA interference (Tet-on shRNA).

Cloning shRNA into pLVET, pLVCT, and pLVPT vectors: first clone shRNA into pLVTHM downstream of the tetO-H1 region. Then cut pLVTHM containing your shRNA with MscI-FspI and clone the insert containing the 3'LTR to target plasmid opened with MscI-FspI. FspI cuts into AmpR. This means for inverted clones AmpR will not be restored; after selection you will be left with clones with the shRNA cassette and functional AmpR.

pLVTHM and packaging plasmid for this system are also available at Addgene (http://www.addgene.org/rnaitools). Please visit Trono lab website (http://tronolab.epfl.ch) to see frequently asked questions on cloning strategies and packaging. You may also visit LentiWeb (http://www.lentiweb.com) for discussion on cloning strategies and protocols.

Addgene has sequenced a portion of this plasmid for verification. Click here for the sequencing result.

Click on map to enlarge

Selected features

HIV-1_5_LTR

465 - 645

truncHIV-1_3_LTR

465 - 645

HIV-1_psi_pack

756 - 800

RRE

1310 - 1543

ORF frame 2

1649 - 2311

cPPT

2042 - 2057

MSCV_rev_primer

2252 - 2229

mPGK_F_primer

2626 - 2645

EGFP_N_primer

2816 - 2795

EGFP

2750 - 3466

ORF frame 2

2750 - 3499

EGFP_C_primer

3403 - 3424

IRES

3550 - 4053

ORF frame 3

4116 - 5123

pBluescriptKS_primer

5209 - 5193

WPRE

5237 - 5824

cPPT

5895 - 5910

U3PPT

5895 - 5916

TRE

5947 - 6234

HIV-1_5_LTR

6270 - 6450

truncHIV-1_3_LTR

6270 - 6450

Sp6_primer

6493 - 6476

pBRrevBam_primer

6802 - 6783

tet(564-300)

6994 - 6731

pGEX_3_primer

7135 - 7157

AmpR_promoter

7316 - 7344

ORF frame 3

7386 - 8246

Ampicillin

7386 - 8246

pBR322_origin

8401 - 9020

pBABE_3_primer

9266 - 9246

SV40_enhancer

9467 - 9252

SV40_promoter

9264 - 9532

SV40_origin

9431 - 9508

SV40_promoter

9384 - 9586

SV40pro_F_primer

9493 - 9512

SV40_int

10713 - 10728

SV40_3_splice

10734 - 10781

SV40_PA_terminator

11357 - 11488

EBV_rev_primer

11445 - 11464

Unique restriction sites

NotI		1155
EagI		1155
BamHI		2704
SmaI		3530
PstI		3538
SacII		5738
MscI		5837
XhoI		5947
XbaI		6454
FspI		7950

Article: A versatile tool for conditional gene expression and knockdown. Szulc J et al. (Nat Methods. 2006 Feb . 3(2):109-16. Pubmed)

Please acknowledge the principal investigator and cite this article if you use this plasmid in a publication.

Also, please include the text "Addgene plasmid 11652" in your Materials and Methods section. This information allows Addgene to create a link from the plasmid page to your publication.