Difference between revisions of "Part:BBa K3332088"

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	'''Fig 1.''' pLtetO-1_RBS1_LacI_terminator_pTrc-2_RBS(B0034)—ecfp-terminator		'''Fig 1.''' pLtetO-1_RBS1_LacI_terminator_pTrc-2_RBS(B0034)—ecfp-terminator
	===Characterization===		===Characterization===
−	The agarose gel electrophoresis images are shown as below:	+	We use pTrc-2 derivative_E0420_pUC57[BBa_K3332087],pLtetO-1_RBS1_lacI_B0015_pTrc-2_E0420_pUC57 and pLtetO-1_RBS1_lacI_B0015_pTrc-2 derivative_E0420_pUC57[BBa_K3332089] to characterize pTrc-2 promoter and pTrc-2 derivative promoter.
		+	The agarose gel electrophoresis images are below:
		+	<table><tr><th>[[File:T--XMU-CHINA--BBa K3332087.png|thumb|500px|'''Fig 2.''' pTrc-2 derivative_E0420_pUC57[BBa_K3332087] digested by ''EcoR'' I and ''Pst'' I (about 1018 bp).]]</th><th></table>
		+	<table><tr><th>[[File:T--XMU-CHINA--BBa K3332088.png|thumb|500px|'''Fig 3.''' pLtetO-1_RBS1_lacI_B0015_pTrc-2_E0420_pUC57[BBa_K3332088] digested by ''Pst'' I (about 5086 bp).]]</th><th></table>
		+	<table><tr><th>[[File:T--XMU-CHINA--BBa K3332089.png|thumb|500px|'''Fig 4.''' pLtetO-1_RBS1_lacI_B0015_pTrc-2 derivative_E0420_pUC57[BBa_K3332089]  digested by ''Pst'' I (about 5125 bp).]]</th><th></table>
−	[[File:T--XMU-CHINA--BBa K3332087.png|none|500px|caption]]	+	'''note:''' E0420 is equal to B0034_E0020_B0015.
−	'''Fig 2.''' pTrc-2 derivative_E0420_pUC57[BBa_K3332087] digested by ''Eco''R I and ''Pst'' I (about 1018 bp)	+
−	[[File:T--XMU-CHINA--BBa K3332088.png|none|500px|caption]]	+
−	'''Fig 3.''' pLtetO-1_RBS1_lacI_B0015_pTrc-2_E0420_pUC57[BBa_K3332088] digested by ''Pst'' I (about 5086 bp)	+
−	[[File:T--XMU-CHINA--BBa K3332089.png|none|500px|caption]]	+
−	'''Fig 4.''' pLtetO-1_RBS1_lacI_B0015_pTrc-2 derivative_E0420_pUC57[BBa_K3332089]  digested by ''Pst'' I (about 5125 bp)	+
−	'''Note：'''E0420 is equal to B0034_E0020_B0015	+	'''Protocol:'''
−	'''Protocol'''	+	1.Preparation of stock solution:dissolve IPTG in absolute alcohol to make 1000× stock solution.
−	1. Preparation of stock solution	+	2.Culture glycerol bacteria containing the corresponding plasmids in test tube for 12h.
−	Dissolve IPTG in absolute alcohol to make 1000× stock solution	+	3.Add 4 mL of the above bacterial solution into 100 mL LB medium and maintain the culture condition at 37 ℃ and 180 rpm.
−	2.Culture glycerol bacteria containing the corresponding plasmid in test tube for 12h.	+	4.Add 100 μL IPTG stock solution into the induction group when OD<sub>600</sub> increased to 0.6.
−		+
−	3.Add 4mL of the above bacterial solution into 100 mL LB medium and maintain the culture condition at 37 ℃ and 180 rpm.	+
−		+
−	4.Add 100μL IPTG stock solution into the induction group when OD increased to 0.6.	+
	5.Induce for 6 hours and the condition is the same as before.		5.Induce for 6 hours and the condition is the same as before.
−	6.Then, sampling 0.5mL culture in each tube. All samples are centrifuged at 12000rpm, 1 minute. Remove supernatant and add 500µL sterile PBS to resuspend.	+	6.Then, sampling 0.5ml culture in each tube. All samples are centrifuged at 12000rpm, 1 minute. Remove supernatant and add 500 µl sterile PBS to resuspend.
−		+
−	7.Measure the fluorescence intensity(ECFP)and corresponding OD600  by 96-well plate reader, then calculate the fluorescence / OD value of each group.	+
		+	7.Measure the fluorescence intensity(ECFP)and corresponding OD<sub>600</sub> by 96-well plate reader, then calculate the fluorescence / OD value of each group.
	Here is the result:		Here is the result:
		+	<html>
		+	<figure>
		+	<img src="https://2020.igem.org/wiki/images/6/6f/T--XMU-China--XMU-China_2020-pTrc2_2d_%E6%8B%BC%E5%9B%BE.png" width="80%" style="float:center">
		+	<figcaption>
		+	<p style="font-size:1rem">
		+	</p>
		+	</figcaption>
		+	</figure>
		+	</html>
		+	'''Fig 5.''' Fluorescence intensity/OD for induction and non-induction group (6 hours). Data are collected and analyzed according to iGEM standard data analysis form．
−	[[File:T--XMU-CHINA--figure 14.png|none|500px|caption]]	+	The strength of pTrc2-derivative and pTrc2 are contrasted. In the figure, pTrc2-derivative are used as the negative control group, pTrc2-derivative_E0420(ECFP) are used as the positive control group while pLtetO-1_LacI_pTrc2_E0420(ECFP) and pLtetO-1_LacI_pTrc2-derivative_E0420(ECFP) are both experimental groups.
−	'''Fig 5.''' Fluorescence intensity/OD600 for induction and non-induction group (6 hours). Data are collected and analyzed according to iGEM standard data analysis form after 6 hours of induction.	+
−		+
−	The strength of pTrc2-derivative and pTrc2 are contrasted. In the figure, pTrc2-derivative are used as the negative control group, the pTrc2-derivative-E0420(ECFP) are used as the positive control group while the pLtetO-1-LacI-pTrc2-E0420 (ECFP) and pLtetO-1-LacI-pTrc2-derivative-E0420(ECFP) are both experimental group.	+
−		+
−	We can see, after adding IPTG to induce the two promoters, the fluorescence intensity are both improved. The change of fluorescence intensity after induction of pLtetO-1-LacI-pTrc2-E0420(ECFP) group is larger than pLtetO-1-LacI-pTrc2-derivative-E0420(ECFP) group, so we can confirm that the LacI has a weak inhibitory effect on pTrc-2 promoter and a strong inhibitory effect on pTrc-2 derivative promoter.	+
−		+
−	[[File:T--XMU-CHINA--pLtetO-1-LacI-pTrc2-E0420.png|none|500px|caption]]	+
−	'''Fig 6.''' In each group，the EP tube on the left is non-induction while the one on the right is induction.	+
−	From this figure, the induction effect can be seen more intuitively.	+	We can see, after adding IPTG to induce the two promoters, the fluorescence intensity are both improved. The change of fluorescence intensity after induction of pLtetO-1-LacI-pTrc2-E0420(ECFP) group is larger than  pLtetO-1-LacI-pTrc2-derivative-E0420(ECFP) group, so we can confirm that LacI has a weak inhibitory effect on pTrc-2 promoter and a strong inhibitory effect on pTrc-2 derivative promoter.
	===Sequence and Features===		===Sequence and Features===
	<partinfo>BBa_K3332088 SequenceAndFeatures</partinfo>		<partinfo>BBa_K3332088 SequenceAndFeatures</partinfo>

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Revision as of 21:00, 27 October 2020

pLtetO-1-RBS1-LacI-ssrAtag(mf-lon)-terminator-pTrc-2-RBS-ECFP-terminator

With this part, the pTrc-2 promoter can be tested by observing the fluorescence intensity.

Usage and Biology

This part can be used to test that if the LacI protein can repress the pTrc-2 promoter. With the expression of LacI, the bacteria have little fluorescence.

Fig 1. pLtetO-1_RBS1_LacI_terminator_pTrc-2_RBS(B0034)—ecfp-terminator

Characterization

We use pTrc-2 derivative_E0420_pUC57[BBa_K3332087],pLtetO-1_RBS1_lacI_B0015_pTrc-2_E0420_pUC57 and pLtetO-1_RBS1_lacI_B0015_pTrc-2 derivative_E0420_pUC57[BBa_K3332089] to characterize pTrc-2 promoter and pTrc-2 derivative promoter. The agarose gel electrophoresis images are below:

Fig 2. pTrc-2 derivative_E0420_pUC57[BBa_K3332087] digested by EcoR I and Pst I (about 1018 bp).

Fig 3. pLtetO-1_RBS1_lacI_B0015_pTrc-2_E0420_pUC57[BBa_K3332088] digested by Pst I (about 5086 bp).

Fig 4. pLtetO-1_RBS1_lacI_B0015_pTrc-2 derivative_E0420_pUC57[BBa_K3332089] digested by Pst I (about 5125 bp).

note: E0420 is equal to B0034_E0020_B0015.

Protocol:

1.Preparation of stock solution:dissolve IPTG in absolute alcohol to make 1000× stock solution.

2.Culture glycerol bacteria containing the corresponding plasmids in test tube for 12h.

3.Add 4 mL of the above bacterial solution into 100 mL LB medium and maintain the culture condition at 37 ℃ and 180 rpm.

4.Add 100 μL IPTG stock solution into the induction group when OD₆₀₀ increased to 0.6.

5.Induce for 6 hours and the condition is the same as before.

6.Then, sampling 0.5ml culture in each tube. All samples are centrifuged at 12000rpm, 1 minute. Remove supernatant and add 500 µl sterile PBS to resuspend.

7.Measure the fluorescence intensity(ECFP)and corresponding OD₆₀₀ by 96-well plate reader, then calculate the fluorescence / OD value of each group. Here is the result:

Fig 5. Fluorescence intensity/OD for induction and non-induction group (6 hours). Data are collected and analyzed according to iGEM standard data analysis form．

The strength of pTrc2-derivative and pTrc2 are contrasted. In the figure, pTrc2-derivative are used as the negative control group, pTrc2-derivative_E0420(ECFP) are used as the positive control group while pLtetO-1_LacI_pTrc2_E0420(ECFP) and pLtetO-1_LacI_pTrc2-derivative_E0420(ECFP) are both experimental groups.

We can see, after adding IPTG to induce the two promoters, the fluorescence intensity are both improved. The change of fluorescence intensity after induction of pLtetO-1-LacI-pTrc2-E0420(ECFP) group is larger than pLtetO-1-LacI-pTrc2-derivative-E0420(ECFP) group, so we can confirm that LacI has a weak inhibitory effect on pTrc-2 promoter and a strong inhibitory effect on pTrc-2 derivative promoter.

Sequence and Features

Reference

[1] Chan CT, Lee JW, Cameron DE, Bashor CJ, Collins JJ. 'Deadman' and 'Passcode' microbial kill switches for bacterial containment. Nat Chem Biol. 2016;12(2):82-86. doi:10.1038/nchembio.1979