Last data update: 24 January 2024 16:39 CET
Plasmid name: pLenti6-strep-hMLKL(211-471)-L291P-Flag puro (LMBP 9168)
New search | Print data sheet |
Price category: | Cat. 1 (cf. price list) |
Status: | GeneCorner non-core plasmid |
Depositor's sequence: | p9168.gb |
Sequence analysis results Genecorner: |
- |
Cloned DNA: |
Human mixed lineage kinase domain like pseudokinase cDNA (MLKL, GeneID 197259); mutated fragment Strep-tag II; N-terminal FLAG epitope tag; C-terminal |
Promoter: | Rous sarcoma virus/human immunodeficiency virus hybrid long terminal repeat (RSV/HIV-1 5' LTR) Human cytomegalovirus immediate early promoter (CMV-IE) and enhancer Escherichia coli lac operon promoter Simian virus 40 early promoter (SV40 early) Phage T3 promoter Phage T7 gene 10 promoter (T7g10) |
Ribosome binding site: |
- |
Terminator: | Rous sarcoma virus/human immunodeficiency virus hybrid long terminal repeat (RSV/HIV-1 3' LTR); modified HIV-1 3' LTR with deleted U3 region (ΔU3/3' LTR) Simian virus 40 polyadenylation signal (SV40 polyA) |
Selection marker: | Ampicillin (amp) Puromycin (puro) |
Replicon: | Escherichia coli plasmid pMB1 origin Phage f1 origin Simian virus 40 bidirectional origin (SV40) |
Host range: | Escherichia coli Mammalian cells; SV40 permissive cells |
Parental clone: | pENTR3C-strep-hMLKL(211-471)-L291P; pLenti6-Flag puro |
Further information: | This lentiviral Gateway expression vector was constructed by cloning the Strep II-tagged mutated human MLKL fragment from pENTR3C-strep-hMLKL(211-471)-L291P into the pLenti6-Flag puro vector. The plasmid encodes for a mutated fragment of the human MLKL gene, consisting of codons 211 up to and including 471, and containing an L291P mutation. The U3 region of the HIV-1 3' LTR is deleted (ΔU3 or dU3) and facilitates self-inactivation of the HIV-1 5' LTR after transduction to enhance the biosafety of the vector. The element also contains a polyadenylation signal for transcription termination and polyadenylation of mRNA in transduced cells. The vector contains the psi packaging signal, allowing viral packaging, and the rev response element (RRE) from HIV-1, permitting Rev-dependent nuclear export of unspliced viral mRNA. Because of the high risk for recombination, plasmid integrity should be checked via PvuII restriction digest after each subcultivation. Because the risk for recombination after each subcultivation is high, this plasmid is only available under the format of isolated plasmid DNA. Other name of the plasmid is pLenti6(puro)-FLAG-dest-strep-hMLKL(211-471)-L291P-stop. |
EMBL Accession number: | - |
Latest sequence update: | 28/04/2017 |
Authenticity test: | The plasmid still needs to be subjected to the authenticity test. |
Class: | Recombinant plasmid |
Type: | Plasmid |
History of deposit: | This plasmid was deposited by Prof. Dr P. Vandenabeele(1) (2). (1) Center for Inflammation Research, VIB, Ghent, Belgium (2) Department of Biomedical Molecular Biology, Ghent University, Ghent, Belgium |
Plasmid reference: | - |
Related plasmid reference: | De Groote et al., BioTechniques 60 (2016), 252-259 [PMID: 27177818] [DOI: 10.2144/000114417] |
Restricted distribution: | - BCCM MTA |
Distributed as: | plasmid DNA |
Host for distribution: | Escherichia coli K12 DH5α |
Host reference: | Focus 8 (1986), 9 |
Related host reference: | Woodcock et al., Nucleic Acids Res. 17 (1989), 3469-3478 [PMID: 2657660] Rodriguez-Quinones et al., Focus 15 (1993), 110-112 Hanahan, J. Mol. Biol. 166 (1983), 557-580 [PMID: 6345791] [DOI: 10.1016/s0022-2836(83)80284-8] Hanahan, in 'DNA Cloning: A Practical Approach Volume I', IRL Press, Oxford (1985), 109-135 [ISSN/ISBN: 0947946187] Grant et al., Proc. Natl. Acad. Sci. U.S.A. 87 (1990), 4645-4649 [PMID: 2162051] |
Cultivation medium: | LB-Lennox + ampicillin (100 μg/ml) |
Cultivation temperature: | 28°C |
Biosafety level: | L1 in E. coli; L2 in mammalian cells |
Other culture collection numbers: | - |
Refer in your Materials and Methods: |
pLenti6-strep-hMLKL(211-471)-L291P-Flag puro (LMBP 9168) is available at BCCM/GeneCorner. This plasmid was deposited by Prof. Dr P. Vandenabeele . |
Note: Up-to-date, validated data are enclosed with the biological material. Nevertheless, these data are a snapshot at a given moment; further updates are always possible.