Protein Purification 2012
DOI: 10.5772/31078
|View full text |Cite
|
Sign up to set email alerts
|

Purification Systems Based on Bacterial Surface Proteins

Help me understand this report

Search citation statements

Order By: Relevance

Paper Sections

Select...
3
1

Citation Types

0
15
0

Year Published

2013
2013
2019
2019

Publication Types

Select...
6

Relationship

2
4

Authors

Journals

citations
Cited by 7 publications
(15 citation statements)
references
References 284 publications
(393 reference statements)
0
15
0
Order By: Relevance
“…Albumin-binding regions spanning one or several albumin-binding domains, for example BB and ABP [22] that are indicated in Figure 1, have been used for affinity purification or depletion of albumin [21]. Moreover, the use of an albumin-binding region as a fusion tag can facilitate affinity purification of a target protein, improve its solubility or be used for directed immobilization [22–24].…”
Section: Introductionmentioning
confidence: 99%
“…Albumin-binding regions spanning one or several albumin-binding domains, for example BB and ABP [22] that are indicated in Figure 1, have been used for affinity purification or depletion of albumin [21]. Moreover, the use of an albumin-binding region as a fusion tag can facilitate affinity purification of a target protein, improve its solubility or be used for directed immobilization [22–24].…”
Section: Introductionmentioning
confidence: 99%
“…A). The advantages of choosing the ZZ‐peptide as a fusion protein include its small size, simple folding structure, high aqueous solubility, and the strong affinity for the Fc‐region of IgGs—a characteristic of Protein A itself (Boström et al, ; Braisted and Wells, ; Jendeberg et al, ). Consequently, the FAP‐ZZ reagents were expressed in Escherichia coli and purified via affinity chromatography utilizing the N‐terminal 6‐histidine tag (A).…”
Section: Resultsmentioning
confidence: 99%
“…2 Protein A chromatography is a simple and highly selective method relying on the strong and specific interaction between Protein A and the crystallizable fragment (Fc) of the antibody. 3,4 Due to this, high yields and exceptional purity can be achieved. Alternatives to Protein A have been explored, such as cation exchange, [5][6][7][8] and nonchromatographic methods like precipitation, [9][10][11] but they have not been able to compete with the well-established Protein A platform when applied to industrial-scale bioprocessing.…”
Section: Introductionmentioning
confidence: 99%
“…Coupling degree (M)*Column volume 3. Number of binding domains per multimer 4. Amount eluted IgG/Molecules per column 5.…”
mentioning
confidence: 99%