The pMAL-c6T Vector provides a method for producing a protein expressed from a cloned gene or open reading frame. The cloned gene is inserted downstream from the malE gene of E. coli, which encodes maltose-binding protein (MBP), resulting in the expression of an MBP fusion protein in the cytoplasm (1,2). The MBP has been engineered for tighter binding to amylose resin. The method uses the strong “tac” promoter and the malE translation initiation signals to give high-level expression of the cloned sequences (3,4), and a one-step purification of the fusion protein using MBP’s affinity for maltose (5). The vector expresses an N-terminal hexahistidine tagged malE gene (lacking its secretory signal sequence) followed by a multiple cloning site containing a TEV protease recognition sequence and stop codons in all three frames. This allows MBP to be cleaved from the protein of interest by TEV Protease after purification. The vector also carries the lacIq gene, which encodes for the Lac repressor. This keeps expression from Ptac low in the absence of IPTG induction.Source: NEB-10 beta competent E. coli (pMAL-c6T)Figure 1: pMAL-c6T VectorThe pMAL- c6T Vector has an exact deletion of the malE signal sequence. Arrows indicate the direction of transcription. Unique restriction sites in the multiple cloning site (MCS) are indicated.
Product Source
NEB-10 beta competent E. coli (pMAL-c6T)
This product is related to the following categories:
NEBExpress MBP Fusion and Purification System,
Bacterial E. coli Protein Expression,
DNA Plasmids & Substrates Products,
Protein Expression
This product can be used in the following applications:
Non-T7 Expression,
Target Protein Insolubility ,
Expression of Difficult Proteins,
Protein Expression in E. Coli,
Protein Expression
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