Part:BBa_K4497039
GFP-mCherry-Fc
This part encodes GFP-mCherry-Fc, GFP fused to mCherry and to an Ig antibody Fc domain. The Fc domain dimerizes through disulfide bonds and allows for easy purification using Protein A chromatography.
Design & Cloning
Design
This part is made of the following components:
- IL-11 Signaling Sequence (Part:BBa_K4497003): Signaling Sequence for secretion
- Flag-tag (Part:BBa_K4497012): Flag epitope tag that enables surface expression detection using immunofluorescence labeling
- mEGFP (Part:Bba_K4497034)
- mCherry(Part:Bba_K4497031)
- TEV recognition sequence (Part:Bba_K4497035: TEV cutting site for removing the Fc-domain from mEGFP after purification.
- Fc domain (Part:Bba_K4497036)
Cloning
We received the part in pcDNA3.1 from Prof. Scheller [1]: pcDNA3.1-spIL11R-GFP-Cherry-TEV-Fc
Purification
We expressed GFP-mCherry-Fc in ExpiCHO using the standard expression protocol (8days) in 25mL of media. The protein was purified from the cell supernatant using a Protein A column (iba-lifesciences) as per protocol of the column. Before application to the column the supernatant was dialyzed into Buffer A overnight. After purification relevant collected fractions were analyzed by SDS PAGE. The chosen fractions were pooled, concentrated and frozen using liquid nitrogen. Protein aliquots were kept in a -80 freezer.
Result
Figure 1. SDS Gel of GFP-mCherry-Fc protein purification. Proteins were purified with Protein A columns. Loading samples (L), waste samples (W) and fractions were loaded. The fractions were chosen with chromatography at λ = 280 nm. Reduced (reducing) samplessample using β-Mercaptoethanol and non reduced (oxidizing) protein samples using NEM were loaded. Marker (M) ‘PageRuler Plus Prestained’ was used.
The purification protocol was adapted from Mossner et al. [1], to be performed significantly faster (several months vs 10 days). While our purity is not as high as shown for the longer protocol, the results were fully sufficient for our ligand binding experiments with the MESA system (Part:Bba_K4497017). The yield was around 4mL with 117µg/mL, which provided plenty of protein for our experiments where we worked with 500ng/mL concentrations in cell media. We used 4 of 80 aliquots during our project.
We used the same protocol to purify GFP-Fc and GFP-mCherry-Fc:
- GFP-Fc: Part:Bba_K4497037
- mCherry-Fc: Part:Bba_K4497038
Sequence and Features
- 10INCOMPATIBLE WITH RFC[10]Illegal XbaI site found at 2182
- 12INCOMPATIBLE WITH RFC[12]Illegal NotI site found at 1576
- 21INCOMPATIBLE WITH RFC[21]Illegal BamHI site found at 94
- 23INCOMPATIBLE WITH RFC[23]Illegal XbaI site found at 2182
- 25INCOMPATIBLE WITH RFC[25]Illegal XbaI site found at 2182
Illegal AgeI site found at 102 - 1000COMPATIBLE WITH RFC[1000]
None |