Difference between revisions of "Part:BBa K1033903"

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'''iGEM2013 Uppsala:''' The images above show ''E coli'' constitutively expressing the chromoproteins amilCP <partinfo>BBa_K592009</partinfo> and tsPurple <partinfo>BBa_K1033906</partinfo> from the high copy plasmid pSB1C3 from the promoters J23116 and J23110.
 
'''iGEM2013 Uppsala:''' The images above show ''E coli'' constitutively expressing the chromoproteins amilCP <partinfo>BBa_K592009</partinfo> and tsPurple <partinfo>BBa_K1033906</partinfo> from the high copy plasmid pSB1C3 from the promoters J23116 and J23110.
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===Contribution===
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Group: Linkoping_Sweden iGEM 2021
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<br>
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Author: Ewelina Bladh
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<br>
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Summary:
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In this contribution, we recorded color development in colonies of ''E.coli'' cells of strain XL1. In addition to studying the color development, we determined tsPurple's absorbance maximum wavelength.<br> <br>
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'''Color Development''' <br>
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In order to determine the progression of color development in colonies, ''E.coli'' cells (XL1) were plated onto LB-Miller agar plates containing a concentration of 25 ug/mL chloramphenicol. The cells were plated in two ways after transformation. The first by plating 100 µL immediately from the liquid culture. The second by first centrifuging the culture, discarding 90% of the supernatant and resuspending the cell pellet in the remaining 10%, followed by plating 100 µL of the resuspension. This results in what is from now on referred to as the diluted and concentrated plate, respectively. <br>
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These plates were incubated in 37°C for the following four days, where they were checked upon each day. ''Figure 1'', displayed below, shows the diluted and concentrated plates of tsPurple during this four day study. The illustration of the diluted plate shows that after 12 hours, no color can be seen to the naked eye. This changes over the course of the next 24 hours, where at 36 hours the colonies on the concentrated plate are clearly visible. The diluted plate appears to need more time to properly express tsPurple, and colonies are not clearly visible until 60 hours after plating. The color intensity continually increases after the first notion of color in the colonies. Additionally, the concentrated plate shows indications of colored colonies already at 12 hours. <br>
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[[Image:Diltspurpleplate.png|800px|center|]]
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[[Image:Tspurpleplate.png|800px|center|]]
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<div class="figurtext" style=font-size:90%;>''Figure 1.'' Top shows the diluted plate over the course of four days. Bottom image shows the concentrated plate over the course of four days. The time each picture was taken after plating is displayed under the each picture in hours.</div> <br>
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'''Absorbance and Fluorescence'''<br>
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Single colonies displaying a purple color were picked from the diluted plates to create liquid cultures. The liquid cultures consist of 5 mL LB-Miller media and a concentration of 25 µg/mL chloramphenicol. The liquid cultures were incubated at 37°C and 200 rpm for the next two days to ensure protein expression. After incubation, the liquid cultures were centrifuged until a pellet formed. The supernatant was discarded, and the remaining pellet was placed in a -20°C freezer. Cell lysis was done using both water and sonication. The frozen pellet was thawed and 5 mL autoclaved dH<sub>2</sub>O was added, followed by vortex treatment to resuspend the pellet. Sonication on ice was the next step taken to lyse any cells that did not lyse upon the addition of water. The amplitude of the sonicator was set to 30%, 30 seconds pulsing followed by 30 seconds rest for a total of 2 minutes. Following sonication, the cultures were centrifuged until a pellet formed whereupon the supernatant was transferred to a clean 15 mL Falcon tube and the pellet was discarded. The supernatant of tsPurple can be see  to the left in ''Figure 2''. Simultaneous experiments with other chromoproteins was also made, their supernatant can be seen with tsPurple to the right in ''Figure 2''. The following chromoproteins were also assessed in the same way as tsPurple: meffBlue (<partinfo>BBa_K1033900</partinfo>), amajLime (<partinfo>BBa_K1033914</partinfo>), spisPink (<partinfo>BBa_K1033923</partinfo>), gfasPurple (<partinfo>BBa_K1033917</partinfo>), and asPink (<partinfo>BBa_K1033926</partinfo>). <br>
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As a control, plates were also made with untransformed XL1-cells. A colony was picked from the diluted plate to start a liquid culture, followed by lysis like the cells transformed with tsPurple. Treatment of control and experimental cells was identical apart from the control culture not being exposed to antibiotics. The supernatant of the control can be seen to the right in ''Figure 2'' along with other chromoproteins. <br>
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[[Image:Tspurple.png|315px|]]
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[[Image:Chromoproteinssupernat.png|550px|]]
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<div class="figurtext" style=font-size:90%;> ''Figure 2.'' To the left, the supernatant of lysed XL1-cells expressing tsPurple following sonication. To the right, all chromoproteins simultaneously experimented on including the control. The chromoproteins pictured to the right, from left to right, are: asPink (<partinfo>BBa_K1033926</partinfo>), gfasPurple (<partinfo>BBa_K1033917</partinfo>), spisPink (<partinfo>BBa_K1033923</partinfo>), meffBlue (<partinfo>BBa_K1033900</partinfo>), tsPurple (<partinfo>BBa_K1033903</partinfo>), amajLime (<partinfo>BBa_K1033914</partinfo>), and the control.  </div> <br>
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In order to measure the absorbance, 100 µL supernatant of tsPurple and 100 µL supernatant of the control were pipetted into a 96-well plate and measurements were made with BMG Clariostar plate reader. Measurements of absorbance were taken every 2 nm in the range 300 nm to 850 nm. This interval was chosen to include the entire visual spectra including margins. The data yielded from the measurements were subsequently baselined by subtracting the control's absorbance values from tsPurple's absorbance values followed by normalization. The resulting graph for tsPurple's absorbance can be seen in ''Figure 3'' below. The absorbance maximum of tsPurple proved to occur at approximately 580 nm. <br>
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[[Image:Tspurpleabs.png|700px|center|]]
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<div class="figurtext" style=font-size:90%;> ''Figure 3.'' Normalized absorbance of tsPurple where the control's absorbance have been subtracted. The absorbance maximum occurs at approximately 580 nm. </div>  <br>
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When examining the supernatant extracted from tsPurple-expressing cells on a UV-table, no fluorescence was detected. The chromoprotein amajLime (<partinfo>BBa_K1033914</partinfo>) was studied at the same time, functioning as a positive control, and the lysate from the control functioned as a negative control.  <br> <br>
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Revision as of 19:56, 19 October 2021

tsPurple, purple chromoprotein (incl RBS, J23110)

This chromoprotein (also known as TinselPurple) naturally exhibits strong color when expressed.

Usage and Biology

This part is useful as a reporter.

AmilCP and tsPurple.jpg

iGEM2013 Uppsala: The images above show E coli constitutively expressing the chromoproteins amilCP BBa_K592009 and tsPurple BBa_K1033906 from the high copy plasmid pSB1C3 from the promoters J23116 and J23110.

Contribution

Group: Linkoping_Sweden iGEM 2021
Author: Ewelina Bladh
Summary: In this contribution, we recorded color development in colonies of E.coli cells of strain XL1. In addition to studying the color development, we determined tsPurple's absorbance maximum wavelength.

Color Development
In order to determine the progression of color development in colonies, E.coli cells (XL1) were plated onto LB-Miller agar plates containing a concentration of 25 ug/mL chloramphenicol. The cells were plated in two ways after transformation. The first by plating 100 µL immediately from the liquid culture. The second by first centrifuging the culture, discarding 90% of the supernatant and resuspending the cell pellet in the remaining 10%, followed by plating 100 µL of the resuspension. This results in what is from now on referred to as the diluted and concentrated plate, respectively.

These plates were incubated in 37°C for the following four days, where they were checked upon each day. Figure 1, displayed below, shows the diluted and concentrated plates of tsPurple during this four day study. The illustration of the diluted plate shows that after 12 hours, no color can be seen to the naked eye. This changes over the course of the next 24 hours, where at 36 hours the colonies on the concentrated plate are clearly visible. The diluted plate appears to need more time to properly express tsPurple, and colonies are not clearly visible until 60 hours after plating. The color intensity continually increases after the first notion of color in the colonies. Additionally, the concentrated plate shows indications of colored colonies already at 12 hours.

Diltspurpleplate.png
Tspurpleplate.png
Figure 1. Top shows the diluted plate over the course of four days. Bottom image shows the concentrated plate over the course of four days. The time each picture was taken after plating is displayed under the each picture in hours.


Absorbance and Fluorescence
Single colonies displaying a purple color were picked from the diluted plates to create liquid cultures. The liquid cultures consist of 5 mL LB-Miller media and a concentration of 25 µg/mL chloramphenicol. The liquid cultures were incubated at 37°C and 200 rpm for the next two days to ensure protein expression. After incubation, the liquid cultures were centrifuged until a pellet formed. The supernatant was discarded, and the remaining pellet was placed in a -20°C freezer. Cell lysis was done using both water and sonication. The frozen pellet was thawed and 5 mL autoclaved dH2O was added, followed by vortex treatment to resuspend the pellet. Sonication on ice was the next step taken to lyse any cells that did not lyse upon the addition of water. The amplitude of the sonicator was set to 30%, 30 seconds pulsing followed by 30 seconds rest for a total of 2 minutes. Following sonication, the cultures were centrifuged until a pellet formed whereupon the supernatant was transferred to a clean 15 mL Falcon tube and the pellet was discarded. The supernatant of tsPurple can be see to the left in Figure 2. Simultaneous experiments with other chromoproteins was also made, their supernatant can be seen with tsPurple to the right in Figure 2. The following chromoproteins were also assessed in the same way as tsPurple: meffBlue (BBa_K1033900), amajLime (BBa_K1033914), spisPink (BBa_K1033923), gfasPurple (BBa_K1033917), and asPink (BBa_K1033926).

As a control, plates were also made with untransformed XL1-cells. A colony was picked from the diluted plate to start a liquid culture, followed by lysis like the cells transformed with tsPurple. Treatment of control and experimental cells was identical apart from the control culture not being exposed to antibiotics. The supernatant of the control can be seen to the right in Figure 2 along with other chromoproteins.

Tspurple.png Chromoproteinssupernat.png

Figure 2. To the left, the supernatant of lysed XL1-cells expressing tsPurple following sonication. To the right, all chromoproteins simultaneously experimented on including the control. The chromoproteins pictured to the right, from left to right, are: asPink (BBa_K1033926), gfasPurple (BBa_K1033917), spisPink (BBa_K1033923), meffBlue (BBa_K1033900), tsPurple (BBa_K1033903), amajLime (BBa_K1033914), and the control.

In order to measure the absorbance, 100 µL supernatant of tsPurple and 100 µL supernatant of the control were pipetted into a 96-well plate and measurements were made with BMG Clariostar plate reader. Measurements of absorbance were taken every 2 nm in the range 300 nm to 850 nm. This interval was chosen to include the entire visual spectra including margins. The data yielded from the measurements were subsequently baselined by subtracting the control's absorbance values from tsPurple's absorbance values followed by normalization. The resulting graph for tsPurple's absorbance can be seen in Figure 3 below. The absorbance maximum of tsPurple proved to occur at approximately 580 nm.

Tspurpleabs.png
Figure 3. Normalized absorbance of tsPurple where the control's absorbance have been subtracted. The absorbance maximum occurs at approximately 580 nm.

When examining the supernatant extracted from tsPurple-expressing cells on a UV-table, no fluorescence was detected. The chromoprotein amajLime (BBa_K1033914) was studied at the same time, functioning as a positive control, and the lysate from the control functioned as a negative control.


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal NheI site found at 7
    Illegal NheI site found at 30
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI.rc site found at 41