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Revision as of 21:14, 17 October 2019
mCherry with hexahistidine tag for purification
This part codes for the red fluorescent protein mCherry with a C-terminal hexahistidine tag for simple purification via metal ions.
Usage and Biology
The red fluorescent protein mCherry was fused to a hexahistidine tag to enable easy purification.
Since the first successful cloning of the green fluorescent protein GFP of Aequorea victoria in 1992
(Prasher et al. 1992) fluorescent proteins became a widely used tool in many fields of research. In contrast to
antibodies labeled with fluorophores that have to cross the cellular membrane which severely disturbes the cellular
integrity, flourescing proteins enable live cell imaging and the investigation of native states of the cell.
Because of the wide range of applications for fluorescing proteins there was a great interest in finding and engineering improved variants and a wider colour spectrum. In the last few years red fluorescing proteins became more and more important. Common native red fluorescing proteins are often dimeric or tetrameric what makes their usage in experimental setups difficult. Directed mutation of dsRFP from the corallimorpharia Discosoma sp. Led to the first monomeric red fluorescing protein mRFP1 (Shaner et al. 2004). Unfortunately this mutations resulted in a lower quantum yield and decreased photostability (Shaner et al. 2004). During further protein engineering attempts, scientists were able to create the red fluorescent protein mCherry. mCherry is a 26.7 kDa protein that shows a very short maturation time of about 15 minutes and a low acid sensitivity. Its excitation maximum lies at 587 nm and it has its emission maxiumum at 610 nm (www.fpbase.org). In 2006 the crystal structure of mCherry was published (Shu and Remington 2006).
Because of the wide range of applications for fluorescing proteins there was a great interest in finding and engineering improved variants and a wider colour spectrum. In the last few years red fluorescing proteins became more and more important. Common native red fluorescing proteins are often dimeric or tetrameric what makes their usage in experimental setups difficult. Directed mutation of dsRFP from the corallimorpharia Discosoma sp. Led to the first monomeric red fluorescing protein mRFP1 (Shaner et al. 2004). Unfortunately this mutations resulted in a lower quantum yield and decreased photostability (Shaner et al. 2004). During further protein engineering attempts, scientists were able to create the red fluorescent protein mCherry. mCherry is a 26.7 kDa protein that shows a very short maturation time of about 15 minutes and a low acid sensitivity. Its excitation maximum lies at 587 nm and it has its emission maxiumum at 610 nm (www.fpbase.org). In 2006 the crystal structure of mCherry was published (Shu and Remington 2006).
Sequence and Features
Sequence was validated by Sanger sequencing
Assembly Compatibility:
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]
Protein purification
The part mCherryHis was expressed, purified and characterized together with the parent part mCherry ( BBa_J06504 ).To further characterize purified mCherry we compared two different purification protocols. Purification via his-tag was compared to the IMPACT-purification protocol from NEB. For this purpose we cloned mCherry ( BBa_J06504 ) into the purification and expression vector pTXB1 from NEB and at the same time added six histidines to the C-terminus of mCherry in pSB1C3 ( BBa_K2926048 ). Both expression vectors were transformed in E. coli ER2566. After induction with IPTG both cultures showed the characteristic red colour of mCherry expressing bacteria (Fig. 2 and Fig. 3).
The expression culture of mCherry in pTXB1 showed a brighter red colour which indicated a higher expression level.
Purification
After cultivation and cell lysis via Ribolyzer the protein was purified using the His-purification kit from Macherey Nagel and the IMPACT-purification kit from NEB (Fig. 4).
A performed Bradford assay showed that expression and purification using the IMPACT-Kit resulted in a higher yield since
we were able to purify 985 µg mCherry from a cell mass of 2.13 g compared to 39.4 µg mCherryHis from a cell mass of 1.92 g.
Both purification methods were analyzed on a SDS-PAGE (Fig. 5).
The SDS-PAGE shows an intense band at the estimated height of around 27 kDa in every lane. This indicates that mCherry
as well as mCherryHis have successfully been expressed. The bands in the wash- and flow-through-fraction show, that not
all of the protein efficiently binds to the purification columns.
In the last lane you can see that we were able to purify mCherry as well as mCherryHis. While the IMPACT-purification resulted in a higher yield, the purity of mCherryHis was higher as the protein lane in Fig. 5 indicated.
Following the SDS-PAGE we analyzed the purified protein via MALDI-ToF. For this purpose we excised the marked bands (Fig. 5) from the SDS-PAGE and started a tryptic digestion of the washed gel fragment. Analysis via MALDI-ToF confirmed that we were able to purify mCherry (Fig. 6).
In the last lane you can see that we were able to purify mCherry as well as mCherryHis. While the IMPACT-purification resulted in a higher yield, the purity of mCherryHis was higher as the protein lane in Fig. 5 indicated.
Following the SDS-PAGE we analyzed the purified protein via MALDI-ToF. For this purpose we excised the marked bands (Fig. 5) from the SDS-PAGE and started a tryptic digestion of the washed gel fragment. Analysis via MALDI-ToF confirmed that we were able to purify mCherry (Fig. 6).
The generated mass spectra and mass lists were evaluated using the software BioTools. To compare the experimentally
determined data to the theoretical protein sequence we performed an in silico trypsine-digestion of the expected protein
sequence and compared the generated mass spectrum and mass list to the measured ones. We were able to match both proteins
to the theoretical spectrum. Additionally we were able to detect the his-tag from mCherryHis in the mass list.
Characterization
To gain some more knowledge about mCherry we analyzed different properties of the protein. First of all we measured its emission- and excitation spectra (Fig. 7).
The resulting spectra show, that adding a his-tag to mCherry does not alter the emission- or excitation spectrum of mCherry.
The excitation maximum of mCherry lies at 587 nm, the emission maximum at 608 nm.
Next we compared the fluorescence intensity of the two different mCherry-variants normalized to Texas Red (Fig. 8).
Next we compared the fluorescence intensity of the two different mCherry-variants normalized to Texas Red (Fig. 8).
The fluorescence intensity of mCherryHis seemed to be higher than the intensity of mCherry purified via IMPACT kit.
This might be due to the different purification protocols. Cleavage of mCherry from the chitin column during the
IMPACT-purification is mediated through incubation of the column for 20-24 h in DTT at room temperature. Those
purification conditions might have a negative impact on the protein. Compared to Texas Red, the fluorescence intensity of
1 µmol mCherryHis equals the fluorescence intensity of 1.92 µmol of the fluorescent dye. In contrast, the fluorescence
intensity of 1 µmol mCherry purified via IMPACT protocol equals the fluorescence intensity of 565 nmol Texas Red.