Difference between revisions of "Team:NAWI Graz/Results"

 
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         <h1>RESULTS</h1>
 
         <h1>RESULTS</h1>
 
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      The following results show that both of our constructs work nearly as expected. The alx-mNeonGreen construct shows, that it can be induced by change from pH 7.0 to pH above 8 and fluorescence was measured 20 minutes after this pH shift. The asr-mCardinal construct was inducible by change from pH 7.0 to pH 5.0 and lower but no fluorescence was detected. The promoter itself was working as expected and we were able to detect the 6xHis-tagged mCardinal protein in cultures at pH 5.0 through a Western Blot.   
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        <h2 class="section-sub">Temperature Sensing</h2>
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    <h2 class="section-sub">pH-Sensing</h2>
 
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    <h3 class="section-sub-sub">Alkaline induced expression</h3>
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            To test if the ibpa promoter actually promotes GFP expression dependent on the temperature, we observed bacterial cultures
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        <p>To test if our pH sensitive constructs express the fluorescence proteins, we cultivated the bacteria hosting the plasmids in LPM with pH 7 overnight. For expression control of our alx-mNeonGreen construct, we inoculated 20 ml LPM with pH 7.0, 8.0 and 8.5 to an OD<sub>600</sub> of 0.2 using the overnight culture. After 20 and 40 minutes 1 ml of each culture was taken and adjusted to the lowest OD<sub>600</sub> of the three samples to standardize the OD<sub>600</sub>. This was necessary as growth at pH 8.0 and 8.5 was significantly slower than at pH 7.0. The diluted samples were used to measure fluorescence (excitation 490 nm, emission 520 nm) and again OD<sub>600</sub> with our plate reader. Three aliquots of each sample were measured (n=3), fluorescence was divided by OD<sub>600</sub> and averages of the three aliquots were taken to obtain the data shown in Figure 1.</p>
            harboring the expression vector at different temperatures over time. Diagram A in figure 1 shows the fluorescence
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            intensity we measured all 15 minutes over 6 hours. Cultivation at 28°C leads to a very slow but steady increase
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            in fluorescence intensity, whereas cultivation at 37°C results in a fast and steady increase in fluorescence
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        <img class="section-image" src="https://static.igem.org/mediawiki/2017/d/dd/Asr_res.png" alt="[Diagramm_alx.xlsx]">
            intensity. For comparison of the different samples, we also divided the value for each sample’s fluorescence
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            intensity by its respective OD600 (= relative fluorescence) to take the cell growth into account. The results
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             <b>Fig 1. Alx controlled mNeonGreen Expression:</b> Culture medium was buffered to pH 7, 8 and 8.5 and inoculated to an OD<sub>600</sub> of 0.2. After 20 and 40 minutes, aliquots were taken and fluorescence (excitation 490 nm, absorbance 520 nm) and OD<sub>600</sub> were measured with the plate reader (n=3).
            are shown in diagram B in figure 1. The bacterial culture showed a decrease in relative fluorescence, when cultivated
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            at 28°C throughout the whole experiment, down to a base level of fluorescence (blue line). When cultivated at
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            37°C, we measured a small decrease for the first hour and afterwards a strong increase of relative fluorescence
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             with time (yellow line). When the temperature was changed to 37°C after three hours of incubation at 28°C, the
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            relative fluorescence started to rise significantly within less than an hour (blue line). When lowered to 28°C
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            from 37°C the intensity of relative fluorescence decreases (grey line).
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          <p>As shown in Fig. 1 fluorescence increases at pH 8.0 and 8.5 at both times compared to a standard culture at pH 7.0. At pH 7.0 cultures still show high fluorescence values with no difference between cultures with our plasmid or cultures without any DNA coding for mNeonGreen (Data not shown). This leads to the conclusion that bacteria on their own emit at ~520 nm when stimulated at 490 nm. Still fluorescence is significantly increased in all cultures at higher pH with a maximum of fluorescence at pH 8.5 after 20 min. This increase in fluorescence allows to distinguish between induced and uninduced. Hence we could show that our <a href="https://2017.igem.org/Team:NAWI_Graz/https://2017.igem.org/Team:NAWI_Graz/pHPlasmid#alx">construct</a> works as planned. The next step would be to test how much base (NaOH) would be needed to change the pH of a defined volume of culture with pH 7.0 to pH 8.5. This data would enable us to use the construct to control the robot. Unfortunately the summer was to short to complete this task.</p>
                <img src="" alt="[temp diagram uno]">
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                <img src="" alt="[temp diagram duo]">
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                <font size="-2">Figure 1:  Change of fluorescence intensity during cultivation in four bacterial cultures. Cultures 1 and 2 were incubated
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                at 28°C and cultures 3 and 4 at 37°C. After 3 hours (red line) the incubation temperature of culture 2 was
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                increased to 37° and the temperature of culture 3 is decreased to 28°C. The excitation wavelength was 485/20
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                nm and the measured emission wavelength was 531/20 nm. A) The measured fluorescence intensity is depicted.
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                B) Relative fluorescence, each measured fluorescence intensity was divided by the measured OD600 of the sample.</font>
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            The change in relative fluorescence with change of temperature indicates that the construct is responding to induction by
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            increase in temperature. When incubated at 37°C, there was a strong increase in overall and relative fluorescence.
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            This result confirms the induction of the ibpa promoter by heat. However, it was also shown that it took some
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            time for the bacteria to adapt to the altered temperature, until a change in fluorescence could be observed.
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            If the culture had already been incubated in the cultivation flask for 3 hours at 28°C, a subsequent rise in
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            temperature to 37°C led to a strong increase in fluorescence within less than an hour. It must be noted though,
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            that the cultivation flasks had to be taken out of the incubator for a short amount of time every 15 minutes
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            to take the samples for the measurement of the fluorescence, which might have interfered with GFP production.
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            To further shorten the time span needed for induction of the ibpa promoter, it would be beneficial to test the
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            expression construct at even higher temperatures. In this case, it would be especially important to keep an eye
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            on cell growth as E. coli wouldn’t tolerate growing under extreme heat shock conditions for an unlimited amount
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            of time. Additionally, in some circumstances it might be possible to further improve the promoter in the future
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            via site-directed mutagenesis. Moreover it could be shown that a decrease in temperature from 37°C to 28°C led
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            to inhibition of the ibpa promoter and consequently the production of fluorescence protein nearly stopped. The
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            reduction of GFP expression happened already shortly after the temperature was reduced, within about 15 minutes.
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            Although the GFP production clearly dropped, when the cultures were incubated at 28°C, there was still a small
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            level of expression. However, in relation to the cell density measured by OD600, the fluorescence significantly
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            decreased. After all, this relative fluorescence acted as the signal that was detected and processed by the associated
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<h3 class="section-sub-sub">Acid induced expression</h3>
 
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         <p>To test acid induced expression of mCardinal controlled by the asr promoter (our asr-mCardinal construct), we tried the same protocol we used for the alx-mNeonGreen but with pH 7.0, 5.0 and 4.5. Unfortunately this did not work out, because, as we discovered later, expression works, but mCardinal, a fluorescence protein with extreme fast maturation time, is designed for expression in mammalian<sup>1</sup> cells and does not show any fluorescence when expressed in <i>E. coli</i>. Therefore we investigated the expression on the protein level with Western blotting. To do so we cultivated bacteria containing the construct overnight in LPM with pH 7.0 and used this culture to inoculate 100 ml LPM with pH 7.0, 5.0 and 4.5 to an OD<sub>600</sub> of 0.1. The cultures were incubated at 37°C. Before inoculating, after 1.5, 2.0 and 2.5 hours 3 OD units were taken of each culture, pelleted and cooled on ice. After all samples were collected they were prepared for SDS gel electrophoresis by sonicating, mixing with loading buffer and heating to 95°C. Samples and pageruler protein standard were <a href="https://2017.igem.org/Team:NAWI_Graz/WP"> separated on a SDS gel and blotted</a> on a nitrocellulose membrane. After washing and incubating with anti-6xHis antibodies tagged with horse radish peroxidase, detection was performed with Thermo Scientific<sup>TM</sup> SuperSignal<sup>TM</sup> West Pico Chemiluminescent Substrate.</p>
 
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        <h2 class="section-sub">pH-Sensing</h2>
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            <b>Fig 2. asr controlled expression of mCardinal:</b> Overlay of the membrane showing the PageRuler prestained protein ladder (S) and a picture showing the signal of the horse radish peroxidase substrate. Lanes from left to right, protein ladder, inoculation culture with pH 7.0, the three samples, pH 7.0, 5.0, 4.5, after 1.5 h (t1), after 2 h (t2) and after 2.5 h (t3).  
<p>To test if our pH sensitive constructs express the fluorescence proteins we cultivated the bacteria hosting the plasmids in LPM with pH 7 overnight. For expression control for our alx-mNeonGreen construct, we inoculated 20ml LPM with pH 7.0, 8.0 and 8.5 to an OD<sub>600</sub> of 0.2 using the overnight culture. After 20 and 40 minutes 1ml of each culture where taken and adjusted to the lowest OD<sub>600</sub> of the three samples to standardize OD<sub>600</sub>. This was necessary growth at pH 8.0 and 8.5 was significant slower than at pH 7.0. This diluted samples where used to measure fluorescence (extinction 490 nm, absorbance 520 nm) and again OD<sub>600</sub> with our plate reader. Three aliquots of each sample where measured (n=3), fluorescence was divided by OD<sub>600</sub> and average of the three aliquots where taken to obtain the data shown in Figure 2.</p>
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              <font size="-2"><b>Figure 2. Alx controlled mNeonGreen Expression: </b>Culture media was bufferd to pH 7, 8 and 8.5 and inoculated to an OD<sub>600</sub> of 0.2. After 20 and 40 minutes, aliquotes where taken and fluorescence (extinction 490 nm, absorbance 520 nm) and OD<sub>600</sub> were measured with the plate reader (n=3).</font><br>
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        <p>All detected signals seen in Fig. 2 are the same height as the 30 kDa band  of the standard, correlating with the size of mCardinal plus TEV-site, f-degron and the 6xHis-tag, with an approximate weight of 29.9 kDa. There is no signal in any sample with pH 7.0 leading to the conclusion that asr is not active at pH 7.0. At pH 5.0 and 4.5 there are bands of different intensity at all time points, hence asr is active at these pH and mCardinal is expressed. This is proof that our construct does work. Also expression is higher at pH 5.0 than at 4.5 especially after 2h (t2) and 2.5 h (t3). To verify these results and use the construct for our robot, a different fluorescence protein can be inserted in the construct and the new construct could be tested and used like the alx construct above.</p>
  
 
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1. Chu, J. et al. Non-invasive intravital imaging of cellular differentiation with a bright red-excitable fluorescent protein. Nature methods 11, 572–578 (2014).
 
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As shown in figure 1. Expression of mNeonGreen is increased at pH 8 and 8.5 compared to standard pH 7. Cultures at ph 7, but also cultures without the mNeonGreen plasmid (data not shown) show a high basic fluorescence, leading to the conclusion that the cells naturally show emission at 520 nm. Still, fluorescence is increased twofold at pH 8.5 after 20 and 40 minutes and fluorescence is significantly increased at pH 8 at both measuring points.</p>
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Latest revision as of 03:29, 2 November 2017

RESULTS

The following results show that both of our constructs work nearly as expected. The alx-mNeonGreen construct shows, that it can be induced by change from pH 7.0 to pH above 8 and fluorescence was measured 20 minutes after this pH shift. The asr-mCardinal construct was inducible by change from pH 7.0 to pH 5.0 and lower but no fluorescence was detected. The promoter itself was working as expected and we were able to detect the 6xHis-tagged mCardinal protein in cultures at pH 5.0 through a Western Blot.

pH-Sensing

Alkaline induced expression

To test if our pH sensitive constructs express the fluorescence proteins, we cultivated the bacteria hosting the plasmids in LPM with pH 7 overnight. For expression control of our alx-mNeonGreen construct, we inoculated 20 ml LPM with pH 7.0, 8.0 and 8.5 to an OD600 of 0.2 using the overnight culture. After 20 and 40 minutes 1 ml of each culture was taken and adjusted to the lowest OD600 of the three samples to standardize the OD600. This was necessary as growth at pH 8.0 and 8.5 was significantly slower than at pH 7.0. The diluted samples were used to measure fluorescence (excitation 490 nm, emission 520 nm) and again OD600 with our plate reader. Three aliquots of each sample were measured (n=3), fluorescence was divided by OD600 and averages of the three aliquots were taken to obtain the data shown in Figure 1.

[Diagramm_alx.xlsx]
Fig 1. Alx controlled mNeonGreen Expression: Culture medium was buffered to pH 7, 8 and 8.5 and inoculated to an OD600 of 0.2. After 20 and 40 minutes, aliquots were taken and fluorescence (excitation 490 nm, absorbance 520 nm) and OD600 were measured with the plate reader (n=3).

As shown in Fig. 1 fluorescence increases at pH 8.0 and 8.5 at both times compared to a standard culture at pH 7.0. At pH 7.0 cultures still show high fluorescence values with no difference between cultures with our plasmid or cultures without any DNA coding for mNeonGreen (Data not shown). This leads to the conclusion that bacteria on their own emit at ~520 nm when stimulated at 490 nm. Still fluorescence is significantly increased in all cultures at higher pH with a maximum of fluorescence at pH 8.5 after 20 min. This increase in fluorescence allows to distinguish between induced and uninduced. Hence we could show that our construct works as planned. The next step would be to test how much base (NaOH) would be needed to change the pH of a defined volume of culture with pH 7.0 to pH 8.5. This data would enable us to use the construct to control the robot. Unfortunately the summer was to short to complete this task.

Acid induced expression

To test acid induced expression of mCardinal controlled by the asr promoter (our asr-mCardinal construct), we tried the same protocol we used for the alx-mNeonGreen but with pH 7.0, 5.0 and 4.5. Unfortunately this did not work out, because, as we discovered later, expression works, but mCardinal, a fluorescence protein with extreme fast maturation time, is designed for expression in mammalian1 cells and does not show any fluorescence when expressed in E. coli. Therefore we investigated the expression on the protein level with Western blotting. To do so we cultivated bacteria containing the construct overnight in LPM with pH 7.0 and used this culture to inoculate 100 ml LPM with pH 7.0, 5.0 and 4.5 to an OD600 of 0.1. The cultures were incubated at 37°C. Before inoculating, after 1.5, 2.0 and 2.5 hours 3 OD units were taken of each culture, pelleted and cooled on ice. After all samples were collected they were prepared for SDS gel electrophoresis by sonicating, mixing with loading buffer and heating to 95°C. Samples and pageruler protein standard were separated on a SDS gel and blotted on a nitrocellulose membrane. After washing and incubating with anti-6xHis antibodies tagged with horse radish peroxidase, detection was performed with Thermo ScientificTM SuperSignalTM West Pico Chemiluminescent Substrate.

[Diagramm_alx.xlsx]
Fig 2. asr controlled expression of mCardinal: Overlay of the membrane showing the PageRuler prestained protein ladder (S) and a picture showing the signal of the horse radish peroxidase substrate. Lanes from left to right, protein ladder, inoculation culture with pH 7.0, the three samples, pH 7.0, 5.0, 4.5, after 1.5 h (t1), after 2 h (t2) and after 2.5 h (t3).

All detected signals seen in Fig. 2 are the same height as the 30 kDa band of the standard, correlating with the size of mCardinal plus TEV-site, f-degron and the 6xHis-tag, with an approximate weight of 29.9 kDa. There is no signal in any sample with pH 7.0 leading to the conclusion that asr is not active at pH 7.0. At pH 5.0 and 4.5 there are bands of different intensity at all time points, hence asr is active at these pH and mCardinal is expressed. This is proof that our construct does work. Also expression is higher at pH 5.0 than at 4.5 especially after 2h (t2) and 2.5 h (t3). To verify these results and use the construct for our robot, a different fluorescence protein can be inserted in the construct and the new construct could be tested and used like the alx construct above.

1. Chu, J. et al. Non-invasive intravital imaging of cellular differentiation with a bright red-excitable fluorescent protein. Nature methods 11, 572–578 (2014).