Part:BBa_K4669027

pET22b(+)_WT-Ferritin

Introducing it to iGEM, we would like to nominate our plasmid pET22b(+)_WT-Ferritin. This plasmid integrates a ready-to-use construct for the expression of the wildtype human heavy chain ferritin in Escherichia coli.

Deletion of restriction recognition sites (RRS)

For contributing the full plasmid to iGEM, we have performed mutagenesis to delete restriction recognition sites for the enzymes BsaI and SapI. Thus, we established a plasmid, compatible with the iGEM regulations and are able to provide the plasmid to future iGEM teams for directly diving into cloning and expression experiments!

With simple PCR mutagenesis, we first deleted one of the RRS and then the other. To confirm the successful deletion of the RRSs, we performed a double digest with both enzymes and run the samples through a 1% agarose gel. As shown in figure 2, the samples with only one deleted RRSs remain higher in the gel due to being linearized by the digest and therefore run slower through the gel than the circular plasmid. The samples with both deletions remains circular and shows a band approximately at the same height as the positive control.

Protein Expression

To express our protein, we transformed E. coli strain BL21(DE) star with our plasmid. Protein production then was induced with 0.25 mM IPTG and incubated the cells at 18 °C for 48 h at 180 rpm. By seperating the proteins in a 15% polyacrylamidgel, we could show that we successfully induced the ferritin expression (Figure 3).

Protein purification

In order to move forward with the subsequent analysis, it was essential that we purify our protein constructs. For this purpose, we used a purification protocol for WT-Ferritin provided by Professor Dr. Tobias Beck.

Our workflow for the purification consisted of heat and ammoniumsulfate precipitation, ion exchange chromatography (IEC), and two size exclusion chromatography (SEC) runs.

To verify if we purified our ferritin, we ran a SDS-PAGE. As you can see in figure 4, the gel only shows one band at the expected height of 21 kDa.

Imaging of ferritin

We were able to show that our expression was fruitful and we were capable to completely purify the ferritin in an IEC, followed by two rounds of SEC. With our purified ferritin container we performed negative staining using Transmission Electron Microscopy (TEM). The pictures of the ferritin protein can be seen in figure 5.

For more information about all of these accomplishments, we invite you to have a look at our results page!

Sequence and Features