Team:XJTLU-CHINA/Description

Chromoprotein is the protein which has conjugeted structure and can express different colors. Since our map was designed to be colorful, experiments aimed to test chromoprotein were needed. At the same time, the color can be used as reporter so that we also use chromoprotein to test other parts in our project.   
There were 3 experiments related to chromoprotein. AeBlue Chromoprotein (BBa_K864401), FwYellow Chromoprotein (BBa_K1033910), amilGFP (BBa_K592010, yellow chromoprotein) and amajLime (BBa_K1033916, green-yellow chromoprotein) were four chromoproteins we used. Firstly, we tested all the chromoprotein we used. Secondly, we combined two chromoproteins together to observe their composite color for our map design. Moreover, LVA tag and AAV tag were added after chromoprotein respectively to examine their function and efficiency of degradation.

For our map design, there are two chromoproteins and one composite chromoprotein mainly for our requirement, yellow, blue and green.  But due to different color of chromoprotein, the test and screen were two necessary steps to choose the fit one to show the nice color.
At the first time, AeBlue Chromoprotein (BBa_K864401) and FwYellow Chromoprotein (BBa_K1033910) were tested respectively with inducible promoters (T7 promoter). The construction is shown in Figure 1. These two parts were assembled on PET 21a plasmid and then transformed into expressible competence E.coli BL21 (DE3). The results were that the growths of bacteria were normal and the colors of these two chromoproteins were distinct.  The result was shown as Figure 2 and Figure 3.

                                      

(Figure 2. The four on the left is Aeblue chromoprotein, and the four on the right is Fw Yellow chromoprotein.)

(Figure 3. These two both are Aeblue blue chromoprotein. The left one is induced under 37 degrees Celsius; the right one is induced under 16 degrees Celsius.)

Next, amilGFP yellow chromoprotein (BBa_K592010), and amajLime green-yellow chromoprotein (BBa_K1033916,) were imported in for further color in our map design. These two parts were linked after constitutive promoter (BBa_J23119) and RBS (BBa_B0034) with assembled on PSB1C3. The construction is shown in Figure 4. Then transformed into E. coli SE 2. The results were that the growths of bacteria were normal and the colors of these two chromoproteins were distinct. See results in Figure 5 and Figure 6.

(Figure 4)

(Figure5. amajLime green-yellow chromoprotein) (Figure 6. amilGFP yellow chromoprotein)

For our map design, green chromoprotein is necessary. Moreover, the changed from green to yellow (Inland) and from green to blue (Coastal) was also important to simulate global warming. Inspired by Paris-Saclay igem team (2014), we combined a yellow chromoprotein and a blue chromoprotein to get green color.
Blue and yellow chromoproteins were assembled together. Two structures were used in Figure 7. The reason why an extra promoter was added after the yellow chromoprotein was to increase the express of blue chromoprotein.

(Figure 7. The construction of expressed Aeblue and Fwyellow chromoprotein together)

The 4ml of liquid medium were used to culture the colony of BL21 (DE 3) for 5 hours, and we use IPTG to induce for 3 hours at 37 degrees centigrade. The result is shown as figure 8. However, what was unexpected was that the final colors of these two were both blue and violent instead of green. It was possible that the yellow color expressed here was not pure yellow. We plan to replace FwYellow chromoprotein.

(Figure 8. The left one is two T7 promoters and one terminator in the plasmid pet 21a. The right one is one T7 promoter and one terminator in the plasmid pet 21a)

In order to improve the color which is blue and violent instead of green, another yellow chromoprotein called amilGFP yellow chromoprotein (BBa_K592010) is brought in our test. The structure we used is shown in Figure 9.

(Figure 9. The construction of expressed Aeblue and amilGFP yellow chromoprotein together)

The 4ml of liquid medium were used to culture the colony of BL21 (DE 3) for 5 hours, and we use IPTG to induce for 12 hours at 16 degrees centigrade. The result is shown as Figure 10. As a result, what was expected was that the final color was green. These two chromoproteins are applied in our map design.

(Figure 10. Three mono-colony expressed both Aeblue and amilGFP yellow chromoprotein)

To perform a smooth color change from the combined green to the single expressed blue/yellow, we’d better shorten the half life of the chromoproteins so that it can quickly disappear after its expression is repressed.

At the beginning spy catcher and spy tag were took into consideration to solve the problem. However, it may overload the host. Then we adopted another method, adding specific oligopeptide to the c-terminal end of the chromoprotein to make it more vulnerable to the attack from endogenous tail-specific proteases. Two tails were chosen for our testing, LVA tag and AAV tag with the sequence RPAANDENYALVA and RPAANDENYAAAV respectively (Andersen et al., 1998). Due to the time limitation, only Aeblue chromoprotein was tested. The construction was shown in Figure 11.

Three groups were used in experiments: AeBlue chromoprotein, AeBlue chromoprotein with AAV tag and AeBlue chromoprotein with LVA tag. Two mono-colonies were chosen from each group. 300ml LB was used to culture the 6 colonies at 37 degrees Celsius for 4 hours. Then 300ul IPTG was added to induce at 16 degrees Celsius for 12 hours. The data was collected from 5 hours to 12 hours, totally 13 points. For each point, 20ml colony liquid was obtained from the 300ml LB culture. 4ml of them was used for OD measurement at 600nm and the rest 16ml of them was used for protein extraction.

Firstly, 16ml bacteria were centrifuged at 6000 rpm for 5 minutes. Then the supernatant was discarded and 10ml PBS was added to resuspend the sediment. After using ultrasonic wave to break the cell, 4ml of mixture was centrifuged at 12000 rpm for 5 minutes. Finally, the absorbance of blue chromoprotein was measured at 597nm by spectrophotometer.

Results are shown as follows.

As shown in the Figure 12, both blue chromoprotein with LVA tail and AAV tail had less accumulation amount than the group of no-tail, which indicated both LVA tail and AAV tail raised the degradation rate. In addition, blue chromoprotein with LVA tail had an even lower accumulation in host cells compared to blue chromoprotein with AAV tail. It was speculated that the LVA tail provided a higher degradation rate. In conclusion, the tails can speed up the degradation of chromoprotein, and LVA tail is highly effective in protein degradation, whereas in our project the AAV tag was chosen to gain a balance between clear color performance and high speed of degradation. Figure 13 shows the color of non-tag, AAV tail and LVA tail after induced 720 minutes.

Anderson,J. (1998) ‘New unstable variants of green fluorescent protein for studies of transient gene expression in bacteria’, Applied and environmental microbiology, 64(6), June, pp.2240-2246.

Chromoprotein is a kind of protein with conjugeted structures and when expressed, it is shown as various colors. Different chromoproteins play a major role in our project as they are essential pigments for us to “draw” a colorful map. Meanwhile, chromoproteins served as reporter when other parts in this project were tested.

Besides white, the original color of E.coli colonies, the global warming map also needs colonies in yellow, blue, and green to represent desert, marine and land areas. Moreover, as this project is a dynamic demonstration of global warming, there should be a balance between the chromoproteins’ degradation and accumulation to make sure one color can appear but later disappear quickly on certain parts of the map. To achieve these goals, 3 experiments have been done. The first two experiments confirmed all the colors needed with naked eyes. The third one showed how the chromoproteins with LVA and AAV tails accumulated in E.coli.

The chromoproteins have been tested are: AeBlue chromoprotein (BBa_K864401), FwYellow chromoprotein (BBa_K1033910), amilGFP (BBa_K592010, yellow) and amajLime (BBa_K1033916, green-yellow).

The results indicated that these exogenous proteins were expressed successfully with little toxic effect on growth of the host bacteria. The expressed color shown in Figure 2 and Figure 3 were also desirable.

There was also an experiment comparing the expression of chromoprotein under different temperature. The Aeblue chromoprotein was tested and in 16 degrees Celsius it gave a deeper color compared to 37 degrees Celsius which may prove that chromoproteins could be better expressed in lower temperature. However, because it is closed to blue when expressed under 37 degrees Celsius, later other experiments were set under this temperature.

Next, amilGFP yellow chromoprotein (BBa_K592010), and amajLime green-yellow chromoprotein (BBa_K1033916,) were further tested as backup for the yellow pigments. We spent time on yellow protein screening rather than blue ones because there were more yellow proteins available from iGem distribution.

These two parts went after a constitutive promoter (BBa_J23119) and RBS (BBa_B0034). Together they were assembled on PSB1C3 and finally transformed into E. coli SE 2. The construction is shown in Figure 4.

The results indicated that these exogenous proteins were expressed successfully with little toxic effect on growth of the host bacteria. The expressed color shown in Figure 5 and Figure 6 were also desirable.

Green is a piece of indispensable composition of a world map, and the changing from green to yellow (Inland) as well as from green to blue (Coastal) are also important to mimic the effect of global warming. Inspired by Paris-Saclay igem team (2014), we combined a yellow chromoprotein and a blue chromoprotein to get green color.

Blue and yellow chromoproteins were designed to express simultaneously. Two different linking methods were illustrated in Figure 7. The reason why an extra promoter was added after the yellow chromoprotein was to increase the expression of blue chromoprotein. Additionally, it enabled us to respectively control to the expression of two chromoproteins. For instance, the green could turn to yellow by repressing the blue chropmoprotein.

The colony of BL21 (DE 3) was cultured in 4ml liquid medium for 5 hours, and induced by IPTG for 3 hours under 37 degree Celsius. The result was shown in figure 8. It was unexpected to see the final colors of the combination were blue and violent instead of green. It was possibly because the yellow color expressed here was not pure yellow. Without pictures kept, the colonies tended to be orange when grown on agar plate. That was why we decided to replace FwYellow chromoprotein with its backups.

The testing of amilGFP yellow chromoprotein (BBa_K592010) is shown in Figure 9.

This time after 5 hours’ culture in 4ml liquid medium, they were induced by IPTG for 12 hours at 16 degrees centigrade. The result is shown as Figure 10. As a result,a desired green color shown. These two chromoproteins would be applied in our map design.

To perform a smooth color change from the combined green to the single expressed blue/yellow, we’d better shorten the half life of the chromoproteins so that it can quickly disappear after its expression is repressed.

At the beginning spy catcher and spy tag were took into consideration to solve the problem. However, it may overload the host. Then we adopted another method, adding specific oligopeptide to the c-terminal end of the chromoprotein to make it more vulnerable to the attack from endogenous tail-specific proteases. Two tails were chosen for our testing, LVA tag and AAV tag with the sequence RPAANDENYALVA and RPAANDENYAAAV respectively (Andersen et al., 1998). Due to the time limitation, only Aeblue chromoprotein was tested. The construction was shown in

Three groups were used in experiments: AeBlue chromoprotein, AeBlue chromoprotein with AAV tag and AeBlue chromoprotein with LVA tag. Two mono-colonies were chosen from each group. 300ml LB was used to culture the 6 colonies at 37 degrees Celsius for 4 hours. Then 300ul IPTG was added to induce at 16 degrees Celsius for 12 hours. The data was collected from 5 hours to 12 hours, totally 13 points. For each point, 20ml colony liquid was obtained from the 300ml LB culture. 4ml of them was used for OD measurement at 600nm and the rest 16ml of them was used for protein extraction.

Firstly, 16ml bacteria were centrifuged at 6000 rpm for 5 minutes. Then the supernatant was discarded and 10ml PBS was added to resuspend the sediment. After using ultrasonic wave to break the cell, 4ml of mixture was centrifuged at 12000 rpm for 5 minutes. Finally, the absorbance of blue chromoprotein was measured at 597nm by spectrophotometer.

Results are shown as follows.

As shown in the Figure 12, both blue chromoprotein with LVA tail and AAV tail had less accumulation amount than the group of no-tail, which indicated both LVA tail and AAV tail raised the degradation rate. In addition, blue chromoprotein with LVA tail had an even lower accumulation in host cells compared to blue chromoprotein with AAV tail. It was speculated that the LVA tail provided a higher degradation rate. In conclusion, the tails can speed up the degradation of chromoprotein, and LVA tail is highly effective in protein degradation, whereas in our project the AAV tag was chosen to gain a balance between clear color performance and high speed of degradation. Figure 13 shows the color of non-tag, AAV tail and LVA tail after induced 720 minutes.

Anderson,J. (1998) ‘New unstable variants of green fluorescent protein for studies of transient gene expression in bacteria’, Applied and environmental microbiology, 64(6), June, pp.2240-2246.