Difference between revisions of "Part:BBa K117002:Experience"

Revision as of 19:50, 5 October 2011

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Applications of BBa_K117002

This promoter is activated indirectly by AI-2 to promote whatever downstream gene ligated behind it.

Characterisation:

For information on characterisation of this new part, please visit Part K117010 Experience and Part K117008 Experience

User Reviews

UNIQa954a743ee8e9402-partinfo-00000000-QINU UNIQa954a743ee8e9402-partinfo-00000001-QINU

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Tokyo Tech 2011

Fluorescence intensity of promoter lsrA-gfp((BBa_K117002)-gfp) was almost the same as promoterless-gfp(negative control).
Strain used in this assay lacks lsrR.
This work is done by Takuya Tsubaki.

This part(BBa_K117002) does not work properly. To confirm this, we introduced a gfp gene(BBa_J54103) downstream of the promoter. As a consequence, fluorescence intensity of lsrA promoter-gfp((BBa_K117002)-gfp) was almost the same as promoterless-gfp(negative control), showing that lsrA promoter(BBa_K117002) does not work properly. In spite of no LsR repression, gene transcription does not take place sufficiently.

We improved this part.Our new lsrA promoter(BBa_K649100) works.

If you want to know why our part works, click [http://2011.igem.org/Team:Tokyo_Tech/Projects/RPS-game/assay#5. here] and visit our team's wiki.

[sample]

Ptet-gfp on pSB1A2(JD22597)

Promoterless-gfp on pSB6A1(JD22597)

PlsrA-gfp on pSB1A2(BBa_K649104)(JD22597)

PlsrA-gfp on pSB1A2(BBa_K11702-gfp)(JD22597)

JD22597 is a strain lacking lsrR.

[Method]

1.Overnight cultures of reporter strains grown at 37 °C in LB medium containing appropriate antibiotics were diluted 1:100 into 3 ml of LB medium and were incubated at 37 °C as fresh cultures.

2. After their OD590 reached 0.15, the fresh cultures were diluted 1:100.

3. After 4-hour incubation at 37 °C, 1 ml of each culture was moved to 1.6ml tube and its fluorescence intensity was measured with a flow cytometer.

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Revision as of 19:47, 5 October 2011 (view source) Yosei (Talk \| contribs) (→‎User Reviews) ← Older edit		Revision as of 19:50, 5 October 2011 (view source) Yosei (Talk \| contribs) (→‎User Reviews) Newer edit →
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	[[Image:lsrA_promoter_activity.png\|thumb\|center\|700px\|Fluorescence intensity of promoter lsrA-gfp((BBa_K117002)-gfp) was almost the same as promoterless-gfp(negative control).<br>Strain used in this assay lacks lsrR.<br>This work is done by Takuya Tsubaki.]]		[[Image:lsrA_promoter_activity.png\|thumb\|center\|700px\|Fluorescence intensity of promoter lsrA-gfp((BBa_K117002)-gfp) was almost the same as promoterless-gfp(negative control).<br>Strain used in this assay lacks lsrR.<br>This work is done by Takuya Tsubaki.]]

−	This part(BBa_K117002) does not work properly. To confirm this, we introduced a gfp gene(BBa_J54103) downstream of the promoter. As a consequence, fluorescence intensity of lsrA promoter-gfp((BBa_K117002)-gfp) was almost the same as promoterless-gfp(negative control), showing that lsrA promoter(BBa_K117002) does not work properly. In spite of no LsR repression, gene transcription does not take place ~~suffuciently~~.	+	This part(BBa_K117002) does not work properly. To confirm this, we introduced a gfp gene(BBa_J54103) downstream of the promoter. As a consequence, fluorescence intensity of lsrA promoter-gfp((BBa_K117002)-gfp) was almost the same as promoterless-gfp(negative control), showing that lsrA promoter(BBa_K117002) does not work properly. In spite of no LsR repression, gene transcription does not take place sufficiently.