Part:BBa_K1189021:Experience
Fusion of ferrtin subunits linked to a DNA detector
Ferritin is a protein shelled nanoparticle and is composed of a mixture of 24 light (BBa_K1189024) and heavy (BBa_K1189025) subunits (see Figure 1). It is ubiquitous across eukaryotic and prokaryotic systems and is used to sequester intracellular iron (Chasteen et al., 1991). The 2013 iGEM Calgary used ferritin’s iron core as a reporter and its protein shell to scaffold a DNA sensing TALE (BBa_K1189022) as part of their project, the FerriTALE. The TALE sequence was based off of BBa_K782004 from the 2012 Slovenia iGEM team. The Calgary team used this TALE as a proof of concept for their DNA detector.
Design features
BBa_K1189021 is a fusion of heavy and light ferritin subunits, such that ferritin nanoparticles are formed from 12 di-subunits. The rationale for this design is that it reduces the number of N-termini on ferritin to which proteins can be fused by half, which is important for lessening potential steric hindrances among the fused TALE in the 3D sphere surrounding ferritin. Additionally, di-subunits mandate a 1:1 ratio of heavy and light subunits, ensuring consistency in ferritin’s iron uptake dynamics. Moreover, these di-subunit fusions have been shown stable in engineered applications with other proteins scaffolded to ferritin (Dehal et al., 2010).
TALE A (BBa_K1189022) is attached to the N-terminus of the ferritin di-subunit. Given that the C-terminus of ferritin is oriented toward the core of ferritin, and that we wanted proteins to be displayed on the outside of the ferritin sphere, we selected the N-terminus (Luzzago et al., 1989). TALE A is connected to ferritin by a flexible GS linker (BBa_1189022). The iGEM Calgary team made this decision because spatial modelling suggested that TALEs require freedom of movement to allow for DNA binding. See Figure two for a diagram of BBa_K1189021.
Results
Performance of BBa_K1189021 as a reporter
BBa_K1189021 was expressed in E. coil BL21 and purified using metal affinity chromatography on an FPLC. The purified protein was chemically modified into Prussian blue ferritin. Output from this TALE-ferritin fusion (BBa_K1189021) was compared to output from ferritin/TALEs bound with a coiled-coil linker (BBa_K1189037).
Purified K_1189021 was successfully converted into Prussian blue ferritin. However, Figure 5 shows that the TALE ferritin fusion is a less effective reporter than ferritin and TALEs connected with coiled-coils linkers (BBa_K1189037). It seems that large protein fusions reduce effectiveness of ferritin as a reporter. Figure 6 shows that ferritin with coiled-coils (BBa_K1189037) maintains reporter functionality when TALEs are scaffolded using coiled-coil linkers. Therefore, the 2013 iGEM Calgary team has elected to use BBa_K1189037 as their FerriTALE DNA detector.
Please see the Prussian blue ferritin Wiki page for a detailed analysis of how Prussian blue ferritin, synthesized from commercially available ferritin, performs as a reporter. This data informs how BBa_K1189037 is useful as a reporter.
User reviews
iGEM Calgary 2013
We expressed and purified this protein from the pSB1C3 cloning vector and isolated a limited amount of product using metal affinity purification and an FPLC (see the large scale expression protocol. We suggest that future teams attempt switching the protein sequence into a low copy number expression vector to improve yield as per our attempt with BBa_K1189037.
References
User Reviews
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