Difference between revisions of "Part:BBa K3506036"

 
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<b><font size="3">Usage and Biology</font></b>
 
<b><font size="3">Usage and Biology</font></b>
  
Green fluorescent protein (GFP) is used as a reporter to provide an easily-observed characterization. Clb2 N124aa is the first 124 amino acids of Clb2. In <i>Saccharomyces cerevisiae</i> BY4741, it promotes the degradation of Clb2 during M and G1 phase.
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Green fluorescent protein (GFP) is used as a reporter to provide an easily-observed characterization. Clb2 N124aa is the first 124 amino acids of Clb2. In <i>Saccharomyces cerevisiae</i> BY4741, it promotes the degradation of Clb2 during M and G1 phase[1].
  
 
We fused Clb2 N124aa to GFP at the N-terminal, therefore the green fluorescence will degrade more quickly after expression. Hence, when GFP is used as a reporter to monitor the state of an inducible promoter, it will react more timely and accurately.  
 
We fused Clb2 N124aa to GFP at the N-terminal, therefore the green fluorescence will degrade more quickly after expression. Hence, when GFP is used as a reporter to monitor the state of an inducible promoter, it will react more timely and accurately.  
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<b><font size="3">Design and Properties</font></b>
 
<b><font size="3">Design and Properties</font></b>
  
[[Image:T--BNU-China--clb2 124-cas9.png|400px|border|center]]
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We design a module which fuses Clb2 N124aa to GFP by linker peptide GSGGSG.
  
We constructed a plasmid containing <i>GAL1</i> promoter, Clb2 N124aa (BBa_K3506010) and GFP (BBa_E0040), using it as experimental group. After induced by galactose for 10 hours, <i>Saccharomyces cerevisiae</i> BY4741 were transferred to the SC-ura (glucose) medium. Then the fluorescence intensity was measured every 30 mins by flow cytometry for 5 hours (Figure. 1). After data collection, the protein degradation curve characterized by fluorescence intensity was processed and plotted. As shown in Figure 2, compared with control group, the Clb2 N124aa and GFP fusion protein degrades much faster.
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[[Image:T--BNU-China--clb2-gfp.png|300px|thumb|center|Figure 1. module: Clb2(N124aa)-GFP]]
  
[[Image:T--BNU-China--GFP.png|900px|thumb|center|Figure 1. The expression of GFP in <i>Saccharomyces cerevisiae</i> BY4741]]
 
  
 +
We constructed a plasmid containing <i>GAL1</i> promoter, Clb2 N124aa (BBa_K3506010) and GFP (BBa_E0040), using it as experimental group. After induced by galactose for 10 hours, <i>Saccharomyces cerevisiae</i> BY4741 were transferred to the SC-ura (glucose) medium. As our expected, the plasmid expressed GFP successfully (Figure 2).
 +
 +
[[Image:T--BNU-China--GFP.png|1600px|thumb|center|Figure 2. The expression of GFP in <i>Saccharomyces cerevisiae</i> BY4741]]
 +
 +
Then the fluorescence intensity was measured every 30 minutes by flow cytometry for 5 hours . After data collection, the protein degradation curve characterized by fluorescence intensity was processed and plotted. As shown in Figure 3, compared with control group (only GFP), the Clb2 N124aa and GFP fusion protein degraded much faster.
 +
 +
[[Image:T--BNU-China--K3506010.png|400px|thumb|center|Figure 3. Fuorenscence intensity by time]]
  
[[Image:T--BNU-China--K3506010.png|500px|thumb|center|Figure 2. Fuorenscence intensity by time]]
 
  
 
<b><font size="3">Experimental approach</font></b>
 
<b><font size="3">Experimental approach</font></b>
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1.Clb2 N124aa was amplified by PCR from the <i>Saccharomyces cerevisiae</i> genome using specific primers.
 
1.Clb2 N124aa was amplified by PCR from the <i>Saccharomyces cerevisiae</i> genome using specific primers.
  
2.The pYES2 plasmid (containing <i>GAL1</i> promoter), Clb2 N124aa, and GFP fragment were connected by in-fusion cloning as experimental group.
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2.The pYES2 plasmid (containing <i>GAL1</i> promoter), Clb2 N124aa, and GFP fragment were connected by in-fusion cloning as experimental group. The control group is the pYES2 plasmid only with GFP.
  
 
3.Both experimental group and control group were transformed into <i>E. coli</i> DH5α.
 
3.Both experimental group and control group were transformed into <i>E. coli</i> DH5α.
  
4.The transformed <i>E. coli</i> were grown in 20 mL of LB-amphenicol (100 mg/ml) in an incubator at 37°C, 180 rpm for 12 hours.
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4.The transformed <i>E. coli</i> were grown in 20 mL of LB-amphenicol (100 mg/mL) in an incubator at 37°C, 180 rpm for 12 hours.
  
5.1 ml of bacterial solution was inoculated into LB-amphenicillin (100 mg/ml) medium and incubated at 37°C for 12 hours in the incubator.
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5.1 mL of bacterial solution was inoculated into LB-amphenicillin (100 mg/mL) medium and incubated at 37°C for 12 hours in the incubator.
  
6.Screen for single colonies in LB-amphenicol (100 mg/ml) medium and perform colony PCR to verify the successful transformation.
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6.Screen for single colonies in LB-amphenicol (100 mg/mL) medium and perform colony PCR to verify the successful transformation.
  
 
7.Select the single colony successfully transformed and incubate overnight in a shaker.
 
7.Select the single colony successfully transformed and incubate overnight in a shaker.
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12.Transfer the yeast cell to the SC-ura(galactose) medium.
 
12.Transfer the yeast cell to the SC-ura(galactose) medium.
  
13.After 10 hours, transfer the yeast cell to the SC-ura(glucose) medium. Then measure the fluorescence intensity every one and a half hours by flow cytometry for 5 hours.
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13.After 10 hours, transfer the yeast cell to the SC-ura(glucose) medium. Then measure the fluorescence intensity every 30 minutes by flow cytometry for 5 hours.
  
  
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<font size="4">improve BBa_E0040 </font><br>
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<font size="4">Improve BBa_E0040 </font><br>
 
We imporved [https://parts.igem.org/Part:BBa_E0040 BBa_E0040]
 
We imporved [https://parts.igem.org/Part:BBa_E0040 BBa_E0040]

Latest revision as of 03:32, 28 October 2020


GFP with degradation tag Clb2 N124aa

GFP coupled with Clb2 N124aa is composed of Clb2 N124aa and GFP through Linker. Clb2 N124aa is the first 124 amino acids of Clb2. In Saccharomyces cerevisiae BY4741. Its function is to help the degradation of Clb2 during G1 and M phase. GFP is from 2019 Distribution kit. A linker, “GSGGSG”, was added between Clb2 N124aa and GFP.


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 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 1048


Usage and Biology

Green fluorescent protein (GFP) is used as a reporter to provide an easily-observed characterization. Clb2 N124aa is the first 124 amino acids of Clb2. In Saccharomyces cerevisiae BY4741, it promotes the degradation of Clb2 during M and G1 phase[1].

We fused Clb2 N124aa to GFP at the N-terminal, therefore the green fluorescence will degrade more quickly after expression. Hence, when GFP is used as a reporter to monitor the state of an inducible promoter, it will react more timely and accurately.


Design and Properties

We design a module which fuses Clb2 N124aa to GFP by linker peptide GSGGSG.

Figure 1. module: Clb2(N124aa)-GFP


We constructed a plasmid containing GAL1 promoter, Clb2 N124aa (BBa_K3506010) and GFP (BBa_E0040), using it as experimental group. After induced by galactose for 10 hours, Saccharomyces cerevisiae BY4741 were transferred to the SC-ura (glucose) medium. As our expected, the plasmid expressed GFP successfully (Figure 2).

Figure 2. The expression of GFP in Saccharomyces cerevisiae BY4741

Then the fluorescence intensity was measured every 30 minutes by flow cytometry for 5 hours . After data collection, the protein degradation curve characterized by fluorescence intensity was processed and plotted. As shown in Figure 3, compared with control group (only GFP), the Clb2 N124aa and GFP fusion protein degraded much faster.

Figure 3. Fuorenscence intensity by time


Experimental approach

1.Clb2 N124aa was amplified by PCR from the Saccharomyces cerevisiae genome using specific primers.

2.The pYES2 plasmid (containing GAL1 promoter), Clb2 N124aa, and GFP fragment were connected by in-fusion cloning as experimental group. The control group is the pYES2 plasmid only with GFP.

3.Both experimental group and control group were transformed into E. coli DH5α.

4.The transformed E. coli were grown in 20 mL of LB-amphenicol (100 mg/mL) in an incubator at 37°C, 180 rpm for 12 hours.

5.1 mL of bacterial solution was inoculated into LB-amphenicillin (100 mg/mL) medium and incubated at 37°C for 12 hours in the incubator.

6.Screen for single colonies in LB-amphenicol (100 mg/mL) medium and perform colony PCR to verify the successful transformation.

7.Select the single colony successfully transformed and incubate overnight in a shaker.

8.Extract the plasmids from E.coli and linearize by single enzyme.

9.Transform the plasmids into competent yeast cell and grow it in SC-ura(glucose) medium at a constant temperature of 30°C for 2 days.

10.Screen single colonies by colony PCR to verify successful transformation.

11.Selected colonies were inoculated into the SC-ura(glucose) medium and grown at 30°C for 14-16h in the incubator.

12.Transfer the yeast cell to the SC-ura(galactose) medium.

13.After 10 hours, transfer the yeast cell to the SC-ura(glucose) medium. Then measure the fluorescence intensity every 30 minutes by flow cytometry for 5 hours.


Reference

[1] Hendrickson, C., Meyn, M. A., 3rd, Morabito, L., & Holloway, S. L. (2001). The KEN box regulates Clb2 proteolysis in G1 and at the metaphase-to-anaphase transition. Current biology : CB, 11(22), 1781–1787.


Improve BBa_E0040
We imporved BBa_E0040