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Protein engineering of an IgG-binding domain allows milder elution conditions during affinity chromatography

Gulich, S. (författare)
Uhlén, Mathias (författare)
KTH,Bioteknologi
Hober, Sophia (författare)
KTH,Bioteknologi
 (creator_code:org_t)
2000
2000
Engelska.
Ingår i: Journal of Biotechnology. - 0168-1656 .- 1873-4863. ; 76:03-feb, s. 233-244
  • Tidskriftsartikel (refereegranskat)
Abstract Ämnesord
Stäng  
  • One of the problems in the recovery of antibodies by affinity chromatography is the low pH, which is normally essential to elute the bound material from the column. Here, we have addressed this problem by constructing destabilized mutants of a domain analogue (domain Z) from an IgG-binding bacterial receptor, protein A. In ol-der to destabilize the IgG-binding domain, two protein engineered variants were constructed using site-directed mutagenesis of the second loop of this antiparallel three-helix bundle domain. In the first mutant (Z6C), the second loop was extended with six glycines in order to evaluate the significance of the loop length. In the second mutant (ZL4G), the original loop sequence was exchanged for glycines in order to evaluate the importance of the loop forming residues. Both mutated variants have a lower a-helical content, as well as a lower thermal and chemical stability compared to the parent 2-molecule. The affinity to IgG was slightly lowered in both cases, mainly due to higher dissociation rates. Interestingly, the elution studies showed that most of the bound IgG-molecules could be eluted at a pH as high as 4.5 from columns with the engineered ligands, while only 70% of the bound IgG could be eluted from the matrix with the parent Z as ligand.

Nyckelord

affinity chromatography
immunoglobulin G
protein engineering
protein Z
staphylococcal protein A
4-helix-bundle protein
rop
simulations
resolution
mutations
stability

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Gulich, S.
Uhlén, Mathias
Hober, Sophia
Artiklar i publikationen
Journal of Biote ...
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