Team:Freiburg/Results/Cellfree
Results: Cell-free Expression
The purpose of cell-free expression in the DiaCHIP is to copy DNA templates into protein microarrays on demand. To enable antibody detection with this protein microarray, the single antigen spots have to be covered with a dense layer of antigens. Thus, the expression efficiency of the cell-free system has to be optimized in order to produce a sufficient amount of target proteins within a timespan that is reasonable for preparation of the DiaCHIP in the suggested applications.
One of the key factors influencing expression efficiency is the design of the expression vector. Therefore, we started with the design of a vector based on pSB1C3 that would allow successful cell-free expression (LINK). Additionally, we received the pQE_HA-GFP-12xHis, an expression vector containing a GFP coding sequence from the BIOSS toolbox (LINK), as an external standard that had already performed well in a cell-free expression system. The third vector we used for our experiments was the pBESTlucTM (LINK/MAP) encoding a luciferase for performing the luciferase assay.
However, the most important thing is of course the expression system itself.
We established our own cell-free expression system, the "DiaMIX" based on an E. coli lysate and additionally obtained a commercially available expression kit.We also provide the protocol in order to give future iGEM Teams the possibility to produce their cell-free expression mix in a low-budget version themselves.
First Successful Expression
Before using our DiaMIX in the microfluidic chamber, we performed some initial experiments in vitro in tubes and, at a later time, in well-plates. In the beginning, we weren't able to express anything. This was due to several factors, like the pH value of our mix. It has to be adjusted in the narrow physiological range (between 7 and 8). With only pH paper at hand, this could only be approximated. The pH value is crucial for the solubility of chemicals for the premix. For pH setting, HEPES-KOH and L-Glutamic acid were used. After adjustment of the pH, further parameters were adapted and the source of errors narrowed down. As prime error sources, the preparations of lysate and premix were repeated. The gained experience took care of many errors.
In the end, the reaction premix itself, proved to be our greatest source for errors and prepared once more. Following this, we could record some basal expression indicating that we could now further optimize our system.
Variation of Mg(OAc)2 Concentration
At first, we investigated the influence of magnesium acetate (Mg(OAc)2) on our reaction. In a publication of Kim et al. [REF.] we read about enhancement of cell-free expression by regular addition of small amounts of Mg. We performed expression experiments where reactions were fed with small amounts of Mg(OAc)2 while others were not. The repeated addition of small amounts of magnesium (100 nmol) every 20 minutes during the reaction was found to increase expression levels and was therefore implemented for future experiments. This was done by pipetting 0.5 μl of a 10 μM magnesium acetate solution into the reaction tube whilst keeping it inside the thermomixer. Positive effects towards expression were immediately visible in a subsequently conducted luciferase assay (see figure 2). However, the actual impact of feeding varied a lot in the experiments (LINK zu labjournal), even among reactions with the same components.
Supplying a reaction lasting for at least two hours with additional chemicals every 20 minutes is quite uncomfortable, so we varied the initial concentration of Mg(OAc)2 in the reaction mix. From personal discussions with a leading scientist on the field of cell-free expression, we were adviced to adjust our mix to an concentration of 15-18 mM Mg+. Therefore, we expressed the pBESTlucTM (LINK) with our DiaMIX at concentrations between 12-16 mM to compare the expression via luciferase assay. The result is shown in figure 3 and reveals the optimal initial concentration of Mg(OAc)2 to be 12 mM.
Variation of DNA Concentration
After establishing the ideal concentration of Mg(OAc)2 in our reactions, we further investigated the optimal concentration of DNA added for expression. Again, pBESTlucTM (LINK) was expressed to allow the analysis via luciferase assay in a microplate reader. Triplicates for reactions of 50 µl volumes were set up with amounts of DNA ranging from 1 µg to 5 µg, as well as a negative control without DNA. Luciferase was expressed using the pBESTlucTM vector and a luciferase assay was performed as described in protocols.
The optimal amount of DNA established for further experiments was 2 - 3 µg. To make subsequent reactions more cost-efficient, reactions 2 µg of DNA per 50 µl were used.
Comparison with Commercial Kit
Having optimized our self-prepared, low-budget cell-free expression mix, we compared it to a commercially available kit and thereby were able to make a statement about the functionality of our DiaMIX. As already shown on the main results page we set up an experiment using the pQE_HA-GFP-12xHis vector (LINK). Furthermore, a from this years iGEM team especially for the application designed vector was used that carried a gene for GFP and an N-terminal 10xHis and a Spy-tag on the other side (This sentence does not work...) . Non-coding areas surrounding the GFP gene were optimized for cell free expression. (link) As seen in Figure 6, the DiaMIX shows a higher fluorecence compared to the commercial kit. Even when the higher basal fluorescence is taken into account. This is an effect of the components in the premix. The commercial kit shows an initial drop in fluorescence. This was observed during every measurement and seems to be an fundamental characteristic of the mix that we attributed quenching effects.
Figure 7 shows the performance of our self-designed vector with tha DiaMIX and the commercial mix. As can be observed, the DiaMIX still performs better than the commercial kit. However, the difference is not as obvious as before. This indicates that the DNA does not yet posses an optimal structure for an effective performance in a cell-free system.
This could be due to differences in the 5' upstream sequence which was demonstrated to have great influence on the initiation of transcription. Furthermore, tags in the beginning of the coding sequence also enhance the expression level as shown by Haberstock, S. et al. 1)
Our self-produced DiaMIX performed about as good as the commercial kit as it is shown in figure 6. Compared to the background, an expression time of two hours resulted in a 2-fold increase of relative fluorescence in both systems. The background fluorescence was estimated by the negative control.
Step by Step Validation
iRIf Measurement of Cell-free Expressed GFP
Encouraged by all the promising results that were obtained, we decided to take the next step and broaden the verification methods of our cell-free expressed proteins by using the iRIf technology. We validated cell-free expressed GFP by pipetting a small amount of the reaction directly onto a glass slide with different surfaces. We checked for the detectability of the protein on specific surfaces binding the His-Tag, and on unspecific surfaces.
We were able to detect GFP expressed with the DiaMIX as seen in figure 8. Elaborate results for the iRIf experiments performed with cell-free expressed proteins can be found on the binding on surface results page.
Immobilizing DNA on PDMS
Insert results of immobilizing DNA on PDMS
On-slide Cell-free Expression
The last step towards a final application in the DiaCHIP is the performance of a cell-free expression reaction between the silicone and the glass slide of the microfluidic chamber. Immobilized DNA on the PDMS slide should be transcribed and translated into proteins. Due to time constraints, we were not able to optimize this process. Nonetheless, initial results can be found on this results page.
In-chamber Expression of GFP
Insert results of on-slide expression of GFP
Cell-free Expression of Antigens
Sadly, we could not show binding of the respective antibodies/serum with the iRIf measurement device. This could be due to folding problems of the antigen during cell-free expression. Moreover, the concentration of expressed C. tetani antigen might not have been high enough to be detected by iRIf measurements.