Difference between revisions of "Part:BBa K5387000:Design"

 
Line 2: Line 2:
 
The sequence has been optimized for expression in ''E. coli''.  
 
The sequence has been optimized for expression in ''E. coli''.  
  
Primers for cloning into pET28a(+) between restriction sites NdeI and EcoRI:  
+
The vector used was pET-28a(+), which His-ag we utilized when expressing our protein.
 +
 
 +
Primers for cloning into pET-28a(+) between restriction sites NdeI and EcoRI:  
 
: fwd: 5'-GCGCCATATGGCAACATATAAAGTTAGGG-3'  
 
: fwd: 5'-GCGCCATATGGCAACATATAAAGTTAGGG-3'  
 
: rev: 5'-GCGCGAATTCTTAGATGCTGATGG-3'
 
: rev: 5'-GCGCGAATTCTTAGATGCTGATGG-3'

Latest revision as of 10:31, 29 September 2024

Design Notes

The sequence has been optimized for expression in E. coli.

The vector used was pET-28a(+), which His-ag we utilized when expressing our protein.

Primers for cloning into pET-28a(+) between restriction sites NdeI and EcoRI:

fwd: 5'-GCGCCATATGGCAACATATAAAGTTAGGG-3'
rev: 5'-GCGCGAATTCTTAGATGCTGATGG-3'