Difference between revisions of "Part:BBa K2144008"
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In order to have a final proof we compared our Sortase A7M to the Sortase A from Stockholm using a FRET | In order to have a final proof we compared our Sortase A7M to the Sortase A from Stockholm using a FRET | ||
| − | connecting 5-Carboxytetramethylrhodamin with a LPETG-tag (TAMRA-LPETG) with GGGG-sfGFP (fig. | + | connecting 5-Carboxytetramethylrhodamin with a LPETG-tag (TAMRA-LPETG) with GGGG-sfGFP (fig. 3). We ran this |
reaction for 3h at 30 °C.<br></p> | reaction for 3h at 30 °C.<br></p> | ||
<img class="img-fluid center" | <img class="img-fluid center" | ||
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<p> | <p> | ||
<b> | <b> | ||
| − | Figure | + | Figure 3: |
</b>A FRET-assay of Sortase A from Stockholm and Sortase A7M connecting TAMRA-LPETG and GGGG-mCherry with | </b>A FRET-assay of Sortase A from Stockholm and Sortase A7M connecting TAMRA-LPETG and GGGG-mCherry with | ||
and without 10mM calcium. The ΔRFU refers to the respective negeative control without Sortase. | and without 10mM calcium. The ΔRFU refers to the respective negeative control without Sortase. | ||
Revision as of 20:12, 18 October 2019
Coding sequence for Sortase A with His-tag
Usage
Sortase A is a bacterial enzyme with the ability to break and form new peptide bonds. The key feature of the enzyme is the specific conjugation reaction it carries out, where the enzyme recognizes a specific amino acid sequence, a so called sorting motif (LPXTG motif in the case of S.aureus) and conjugate this sequence with another unit carrying an oligo glycine motif where a new peptide bond is formed [1],[2].
Biology & BioBrick Design
This Biobrick is a truncated version of the enzyme where the transmembrane domain (amino acids 1-59) is not included in the coding sequence to increase solubility [2]. Further, the BioBrick has also been fused with the Protein G B1 Domain (GB1), upstream the Sortase coding sequence, acting as a solubility tag and a His-tag to enabling purification through IMAC [2].
Characterization by iGEM TU_Darmstadt 2019 (Expression and assays)
We purified the Sortase A from team Stockholm via fast protein liquid chromatography (FPLC) using the ÄKTA pure (fig. 2). In order to purify the Sortase A from team Stockholm we used the existing His-tag.
< ----- Bild von ÄKTA Chromatogram ---->Fig 1: Chromatogram of the ÄKTA during the purification of Sortase A from team Stockholm.
In figure 2 it is shown that the Sortase A from Stockholm eluted at ???. This should make sure that we have
purified the right protein with the fitting tag.
We then confirmed the data of the purification by checking on the size of the Sortase using SDS-PAGE (fig. 2).
We purified it twice with the same result in size.
Figure 2: A SDS-PAGE of a triplicate of the reaction solution for the sortase reaction consisting of coat protein (CP), mCherry and Sortase A from Stockholm which were incubated for 90 minutes at 37 °C. A negative control without Sortase A from Stockholm in a triplicate is also included. To verify the size the Sortase A from Stockholm was also put as a control on the gel solely.
In figure 2 a SDS-PAGE of the first sortase reaction performed with the Sortase A from Stockholm is shown as well. On the right is a triplicate of the purified Sortase A from Stockholm to reassure it has the right size of about 15 kDa which is the case. On the left are triplicates of coat protein with an LPETGG-tag (CP-LPETGG) and GGGG-mCherry. The first three are with Sortase Stockholm in the reaction and the middle three are without Sortase Stockholm. The reaction was run at 37 °C for 90 minutes. Seeing this first gel arose the suspicion that the Sortase A from team Stockholm is not working properly.
In order to have a final proof we compared our Sortase A7M to the Sortase A from Stockholm using a FRET connecting 5-Carboxytetramethylrhodamin with a LPETG-tag (TAMRA-LPETG) with GGGG-sfGFP (fig. 3). We ran this reaction for 3h at 30 °C.
Figure 3: A FRET-assay of Sortase A from Stockholm and Sortase A7M connecting TAMRA-LPETG and GGGG-mCherry with and without 10mM calcium. The ΔRFU refers to the respective negeative control without Sortase.
As visible in figure 4 the Sortase A from Stockholm does not show any activity during the reaction although it
was incubated with 10mM calcium present. In contrary to our Sortase A7M which was incubated without calcium
because it is an independent mutant. The Sortase A7M also shows the expected increase in fluorescence visible in
the ΔRFU at 514 nm over time. The ΔRFU refers to the difference between the negative control without the
respective sortase (data not shown). In comparison the Stockholm Sortase A does not seem to catalyze any
reactions over the measured time span. If there would be any activity it would look similar to the graph of the
Sortase A7M where the ΔRFU at 514 nm is increased due to the FRET pair being connected. This confirms the
SDS-PAGEs that showed the same outcome of the Sortase A from Stockholm being not functional independent from the
presence of calcium.
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
References
[1] Popp, M. W.-L. and Ploegh, H. L. (2011), Making and Breaking Peptide Bonds: Protein Engineering Using Sortase. Angew. Chem. Int. Ed., 50: 5024–503
[2] Westerlund, K. Karlstrom, A., Honarvar, H., Tolmachev, V. Design, Preparation, and Characterization of PNA-Based Hybridization Probes for Affibody-Molecule-Mediated Pretargeting. Bioconjugate Chem., 2015, 26 (8), pp 1724–1736