BBa_K1499503

BBa_K1499503 Version 1

Component

Source:

http://parts.igem.org/Part:BBa_K1499503

Generated By: https://synbiohub.org/public/igem/igem2sbol/1

Created by: Aryo Sorayya

Date created: 2014-10-07 11:00:00

Date modified: 2015-05-08 01:10:46

quorum sensing machinery that activates GFP expression with extra terminator

Details

• Types: DnaRegion
• Roles: engineered_region; Composite
• Sequences: BBa_K1499503_sequence (Version 1)

Description

This is the same part as Part:BBa_K1499500, except that it has two more terminators between the luxR gene and the luxPR promoter.

Notes

After ligating the BBa_K1499500 construct together and into the BioBrick backbone, we transformed it into the NEB 5-alpha strain of E. coli. The colonies that fluoresced were most likely to have been successfully transformed, and thus these were sent off for sequencing. The sequencing data showed that our construct was correct (see below), so we were able to submit for BioBricking.


Lux sequencing data.jpg


Although our sequencing data was good, we realized that we had not induced the lac-repressible promoter, and thus the colonies should not have been fluorescing yet. After doing more research, we realized that the strain of E. coli we were using was not lactose deficient, thus the quorum sensing cascade was being activated by the natural presence of lactose. We ordered a lacI^q strain of E. coli, which are lac deficient, so that we could have complete control of GFP expression. However, when we performed the transformation of the construct into this strain, all of the colonies still fluoresced.

After doing further research, we discovered that the luxPR promoter (BBa_R0062) [2], will induce backward transcription if the luxR protein is present but the AHL molecule is not. In the lac deficient strain of E. coli, AHL is not produced without IPTG induction, but luxR expression is controlled by the constitutive ptet promoter. We hypothesize that since luxR was present in these cells without AHL, the backward transcription from luxPR hindered the function of the terminators that separated the luxR gene from the GFP gene. Thus GFP may have been expressed because the ptet promoter, which is constitutive, was able to affect its expression.

In order to bypass this issue, inserted two more terminators between the luxR gene and the luxPR promoter, in hopes that this would stop the backward transcription from having an effect on GFP expression, allowing us to work towards measuring the time delay created by our construct. The double-promoter did help reduce the GFP expression, though not completely.

Source

BBa_K1499500

Components

Access	Instance	Definition
public	BBa_R0011	lacI+pL
public	BBa_B0034	BBa_B0034
public	BBa_C0161	luxI
public	BBa_B0010	BBa_B0010
public	BBa_B0012	BBa_B0012
public	BBa_R0040	p(tetR)
public	BBa_B0034	BBa_B0034
public	BBa_C0062	luxr
public	BBa_B0010	BBa_B0010
public	BBa_B0012	BBa_B0012
public	BBa_B0010	BBa_B0010
public	BBa_B0012	BBa_B0012
public	BBa_R0062	lux pR
public	BBa_B0032	BBa_B0032
public	BBa_E0040	GFP
public	BBa_B0010	BBa_B0010
public	BBa_B0012	BBa_B0012

Sequence Annotations

Sequence Annotation	Location	Component / Role(s)
BBa_R0011	1,54	lacI+pL
BBa_B0034	64,75	BBa_B0034
BBa_C0161	82,666	luxI
BBa_B0010	675,754	BBa_B0010
BBa_B0012	763,803	BBa_B0012
BBa_R0040	812,865	p(tetR)
BBa_B0034	874,885	BBa_B0034
BBa_C0062	892,1647	luxr
BBa_B0010	1681,1760	BBa_B0010
BBa_B0012	1769,1809	BBa_B0012
BBa_B0010	1818,1897	BBa_B0010
BBa_B0012	1906,1946	BBa_B0012
BBa_R0062	1955,2009	lux pR
BBa_B0032	2018,2030	BBa_B0032
BBa_E0040	2037,2756	GFP
BBa_B0010	2765,2844	BBa_B0010
BBa_B0012	2853,2893	BBa_B0012

Other Properties

• igem#experience: Works
• igem#sampleStatus: It's complicated
• igem#status: Planning
• synbiohub#ownedBy: user/james
• synbiohub#ownedBy: user/myers
• synbiohub#topLevel: BBa_K1499503/1

Member of these Collections

• iGEM Parts Registry