pLSG-IBA167 vector

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Insect expression vector encoding an N-terminal FLAG-tag and Twin-Strep-tag®
pLSG-IBA167 vector

The pLSG-IBA167 vector is designed for high-level expression of target proteins with an N-terminal FLAG-tag and Twin-Strep-tag® in insect cells. The gene transfer into the polyhedrin gene locus of AcMNPV DNA is achieved by homologous recombination and the vector carries a polyhedrin promoter. Co-transfection with BacPAK6 linearized AcMNPV DNA (Clontech) or with circular flashBAC modified AcMNPV DNA (Oxford Expression Technologies) allows the generation of recombinant baculovirus at very high efficiency through reconstitution of an essential gene (ORF 1629) and elimination of wild-type virus to great extent. For selection and propagation in E. coli, the vector carries an ampicillin resistance and ColE1 origin of replication (pUC). Please note that cloning into pLSG-IBA Acceptor Vectors compulsorily requires the restriction enzyme Esp3I since no other MCS for the integration of a gene of interest is available. In addition to the direct cloning of the gene of interest into pLSG-IBA vectors with Esp3I, another option via a so-called Entry Vector is possible.

Specifications

  • Cloning Method: Direct cloning using restriction enzyme Esp3I
  • Concentration: 250 ng/µl
  • Expression Host: Insect cells
  • Form: Suspension in TE buffer
  • Possible Application: Vector for recombinant expression in insect cells
  • Promoter: Polyhedrin Promoter
  • Resistance: Ampicillin
  • Sequence: See Documents
  • Size: 6290 bp

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