Difference between revisions of "Part:BBa K1632004"
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<partinfo>BBa_K1632004 short</partinfo> | <partinfo>BBa_K1632004 short</partinfo> | ||
− | [[Image:Tokyo Tech fim switch (wild-type) design.png| | + | [[Image:Tokyo Tech fim switch (wild-type) design.png|thumb|center|400px|Fig. 1. Overview of fim inversion system]]<br> |
− | ''Fim'' switch (wild-type) is derived from wild-type sequence. ''Fim'' switch (wild-type) have sigma 70 promoter which is | + | <span style="margin-left: 10px;">''Fim'' switch(wild-type) is derived from wild-type sequence. ''Fim'' switch(wild-type) have sigma 70 promoter which is constitutive promoter. The promoter in the ''fim'' switch transcripts to the right. From the direction of transcription, the state is defined as [ON] state. On the other hand, fim switch[default OFF](wild-type) (<partinfo>BBa_K1632005</partinfo>) transcripts to the left.<br> |
+ | <span style="margin-left: 10px;">''Fim'' switch is inverted by two recombinase, FimB and FimE. The FimB protein inverts ''fim'' switch from [ON] state to [OFF] state and from [OFF] state to [ON] state with approximately equal efficiencies. On the other hand, the FimE protein inverts ''fim'' switch predominantly from [ON] state to [OFF] state.<br> | ||
− | '' | + | <span style="margin-left: 10px;">We constructed ''fim'' switch[default ON](wild-type)_rbs_''gfp''(<partinfo>BBa_K1632007</partinfo>) to characterize the function of this part, by inserting ''fim'' switch[default ON](wild-type)(<partinfo>BBa_K1632004</partinfo>) upstream of a GFP coding sequence. <br> |
+ | <span style="margin-left: 10px;">In the ''fimB'' dependent ''fim'' switch state assay, we transformed ''fim'' switch[default ON](wild-type)_rbs_''gfp'' and PBAD/''araC''_''fimB''(<partinfo>BBa_K1632012</partinfo>) in the E.coli DH5alpha strain. We measured the fluorescence intensity of the cells induced by arabinose. <br> | ||
+ | [[Image:Tokyo_Tech_FimB_assay_Results.png |thumb|center|700px|<b>Fig. 2. </b>The histograms of the samples measured by the flow cytometer]]<br> | ||
− | We | + | <span style="margin-left: 10px;"><span style="margin-left: 10px;">We tried to confirm that <i>fim</i> switch is bidirectically inverted in the presence of FimB(wild-type) by using GFP as a reporter, under 4 different concentrations of arabinose. In the medium with 0 M arabinose, we supplemented the medium with 0.5 % glucose in order to repress the leakage in the PBAD/''araC'' promoter. Fig. 2 shows the histograms of the samples measured by the flow cytometer. In the results of the reporter cell (1), when the Induction of FimB(wild-type) expression increases, the fluorescence intensity decreases. From this fact, we confirmed that the <i>fim</i> switch is inverted from [ON] state to [OFF] state by FimB(wild-type). From the result of the reporter cell (2), when the expression amount of FimB(wild-type) increases, the expression amount of GFP in the reporter cell (2) increases. From this fact, we confirmed that the <i>fim</i> switch is inverted from [OFF] state to [ON] state by FimB(wild-type). From the results of the two reporter cells (1) and (2), we successfully confirmed that FimB(wild-type) inverts the <i>fim</i> switch from [ON] state to [OFF] state and from [OFF] state to [ON] state.<br> |
− | In the | + | [[Image:Tokyo_Tech_FLA_colony_FimB.png |thumb|center|600px|<b>Fig. 3. </b> Determination of percemtage of [ON] state and colony formation using plasmid mixture extracted cell expressing FimB.]]<br> |
+ | To confirm our results that our FimB(wild-type) inverted the <i>fim</i> switch(wild-type) further, after scattering the samples on a plate, we counted the number of colonies which were expressing GFP and the colonies which were not expressing GFP(Fig.3). The state of <i>fim</i> switch either [ON] or [OFF] in colonies is evaluated from fluorescence. In brief, colonies which contain <i>fim</i> switch[default ON] expresse GFP while colonies which contain <i>fim</i> switch[default OFF] do not express GFP. We counted out the all colonies and colonies which contain <i>fim</i> switch[default ON]. In the results of the reporter cell (1), when the expression of FimB(wild-type) was induced by arabinose, the percentage of [ON] state decreased. Furthermore, from the results of the reporter cell (2), when the expression of FimB(wild-type) was induced, the percentage of [ON] state increased. From the results of the two reporter cells (1) and (2), we successfully confirmed that the FimB protein inverts the <i>fim</i> switch(wild-type) from [ON] state to [OFF] state and from [OFF] state to [ON] state. (Fig.3). This result was consistent with the histograms (Fig. 2)<br> | ||
+ | [[Image:Tokyo_Tech_FImB_sequence.png |thumb|center|600px|<b>Fig. 4. </b> DNA sequencing results of <i>fim</i> switch(wild-type)]]<br> | ||
+ | Also, we incubated the colonies with fluorescence and the colonies without fluorescence. We minipreped cell cultures. Sequence complementarity of the each sample in the specific region of the switch shows intended inversion of the switch from [ON] state to [OFF] state in all samples (Fig. 4.).<br><br><br> | ||
+ | <span style="margin-left: 10px;">Similary,in the fimE dependent ''fim'' switch state assay, we transformed ''fim'' switch[default ON](wild-type)_rbs_''gfp'' and PBAD/''araC''_''fimE''(wild-type)(<partinfo>BBa_K1632013</partinfo>) in the E.coli DH5alfpha strain. We measured the fluorescence intensity of the cells induced by arabinose. <br> | ||
− | + | [[Image:Tokyo_Tech_FimE_assay_Results.png |thumb|center|700px|<b>Fig. 5. </b>The histograms of the samples measured by flow cytometer]]<br> | |
+ | We tried to confirm that <i>fim</i> switch(wild-type) is predominantly inverted in the presence of FimE(wild-type) by using GFP as a reporter, under 4 different concentrations of arabinose. In the medium with 0 M arabinose, we supplemented the medium with 1.0 % glucose in order to repress the leakage in the PBAD/araC promoter. Fig. 5 shows the histograms of the samples measured by the flow cytometer. In the results of the reporter cell (1), when the induction of FimE(wild-type) expression increases, the fluorescence intensity decreases. From this fact, we confirmed that the <i>fim</i> switch(wild-type) is inverted from [ON] state to [OFF] state by FimE(wild-type). From the result of the reporter cell (2), even when the expression amount of FimE(wild-type) increases, the expression amount of GFP in the reporter cell (2) does not change. From this fact, we confirmed that the <i>fim</i> switch(wild-type) is inverted only from [ON] state to [OFF] state by FimE(wild-type). From the results of the two reporter cells (1) and (2), we successfully confirmed that FimE(wild-type) inverts the <i>fim</i> switch(wild-type) only from [ON] state to [OFF] state. | ||
+ | |||
+ | |||
+ | [[Image:Tokyo_Tech_FLA_FImE_.png |thumb|center|700px|<b>Fig. 6. </b>The histograms of the samples measured by flow cytometer]]<br> | ||
+ | After measurement of flow cytometer, we minipreped the cell culture and got plasmid mixture which contain pSB6A1 and pSB3K3 in each sample.The state of <i>fim</i> switch(wild-type) either [ON] state or [OFF] state in colonies is evaluated from fluorescence. Thus, colonies which contain <i>fim</i> switch[default ON](wild-type) expressed GFP. On the other hand, colonies which contain <i>fim</i> switch[default OFF](wild-type) do not express GFP. We counted out the all colonies and those with fluorescence. In the results of the reporter cell (1), when inducing the expression of FimE(wild-type), the percentage of [ON] state decreased dramatically. On the other hand, from the results of the reporter cell (2), when inducing the expression of FimE(wild-type), the percentage of [ON] state remained being small. From the results of the two reporter cells (1) and (2), we successfully confirmed that FimE(wild-type) inverts the <i>fim</i> switch(wild-type) predominantly from [ON] state to [OFF] state. (Fig.6). This result was consistent with the histograms (Fig.5.). | ||
+ | |||
+ | [[Image:Tokyo_Tech_sequence_FimE.png |thumb|center|700px|<b>Fig. 7. </b>The histograms of the samples measured by flow cytometer]]<br> | ||
+ | Also, we incubated the colonies with fluorescence and those without fluorescence. We minipreped cell culture. Sequence complementarity in the specific region of the switch shows intended inversion of the switch from [ON] state to [OFF] state in all sample (Fig.7.). | ||
+ | |||
+ | ===More information=== | ||
+ | |||
+ | For more information, see [[http://2015.igem.org/Team:Tokyo_Tech/Project Our work in Tokyo_Tech 2015 wiki]], [[http://2015.igem.org/Team:Tokyo_Tech/Experiment/ssrA_tag_degradation_assay About ssrA-tag]], [[http://2015.igem.org/Team:Tokyo_Tech/Experiment/Overview_of_fim_inversion_system About ''fim'' inversion system]] | ||
<!-- Add more about the biology of this part here | <!-- Add more about the biology of this part here |
Latest revision as of 03:28, 19 September 2015
fim switch[default ON](wild-type)
Fim switch(wild-type) is derived from wild-type sequence. Fim switch(wild-type) have sigma 70 promoter which is constitutive promoter. The promoter in the fim switch transcripts to the right. From the direction of transcription, the state is defined as [ON] state. On the other hand, fim switch[default OFF](wild-type) (BBa_K1632005) transcripts to the left.
Fim switch is inverted by two recombinase, FimB and FimE. The FimB protein inverts fim switch from [ON] state to [OFF] state and from [OFF] state to [ON] state with approximately equal efficiencies. On the other hand, the FimE protein inverts fim switch predominantly from [ON] state to [OFF] state.
We constructed fim switch[default ON](wild-type)_rbs_gfp(BBa_K1632007) to characterize the function of this part, by inserting fim switch[default ON](wild-type)(BBa_K1632004) upstream of a GFP coding sequence.
In the fimB dependent fim switch state assay, we transformed fim switch[default ON](wild-type)_rbs_gfp and PBAD/araC_fimB(BBa_K1632012) in the E.coli DH5alpha strain. We measured the fluorescence intensity of the cells induced by arabinose.
We tried to confirm that fim switch is bidirectically inverted in the presence of FimB(wild-type) by using GFP as a reporter, under 4 different concentrations of arabinose. In the medium with 0 M arabinose, we supplemented the medium with 0.5 % glucose in order to repress the leakage in the PBAD/araC promoter. Fig. 2 shows the histograms of the samples measured by the flow cytometer. In the results of the reporter cell (1), when the Induction of FimB(wild-type) expression increases, the fluorescence intensity decreases. From this fact, we confirmed that the fim switch is inverted from [ON] state to [OFF] state by FimB(wild-type). From the result of the reporter cell (2), when the expression amount of FimB(wild-type) increases, the expression amount of GFP in the reporter cell (2) increases. From this fact, we confirmed that the fim switch is inverted from [OFF] state to [ON] state by FimB(wild-type). From the results of the two reporter cells (1) and (2), we successfully confirmed that FimB(wild-type) inverts the fim switch from [ON] state to [OFF] state and from [OFF] state to [ON] state.
To confirm our results that our FimB(wild-type) inverted the fim switch(wild-type) further, after scattering the samples on a plate, we counted the number of colonies which were expressing GFP and the colonies which were not expressing GFP(Fig.3). The state of fim switch either [ON] or [OFF] in colonies is evaluated from fluorescence. In brief, colonies which contain fim switch[default ON] expresse GFP while colonies which contain fim switch[default OFF] do not express GFP. We counted out the all colonies and colonies which contain fim switch[default ON]. In the results of the reporter cell (1), when the expression of FimB(wild-type) was induced by arabinose, the percentage of [ON] state decreased. Furthermore, from the results of the reporter cell (2), when the expression of FimB(wild-type) was induced, the percentage of [ON] state increased. From the results of the two reporter cells (1) and (2), we successfully confirmed that the FimB protein inverts the fim switch(wild-type) from [ON] state to [OFF] state and from [OFF] state to [ON] state. (Fig.3). This result was consistent with the histograms (Fig. 2)
Also, we incubated the colonies with fluorescence and the colonies without fluorescence. We minipreped cell cultures. Sequence complementarity of the each sample in the specific region of the switch shows intended inversion of the switch from [ON] state to [OFF] state in all samples (Fig. 4.).
Similary,in the fimE dependent fim switch state assay, we transformed fim switch[default ON](wild-type)_rbs_gfp and PBAD/araC_fimE(wild-type)(BBa_K1632013) in the E.coli DH5alfpha strain. We measured the fluorescence intensity of the cells induced by arabinose.
We tried to confirm that fim switch(wild-type) is predominantly inverted in the presence of FimE(wild-type) by using GFP as a reporter, under 4 different concentrations of arabinose. In the medium with 0 M arabinose, we supplemented the medium with 1.0 % glucose in order to repress the leakage in the PBAD/araC promoter. Fig. 5 shows the histograms of the samples measured by the flow cytometer. In the results of the reporter cell (1), when the induction of FimE(wild-type) expression increases, the fluorescence intensity decreases. From this fact, we confirmed that the fim switch(wild-type) is inverted from [ON] state to [OFF] state by FimE(wild-type). From the result of the reporter cell (2), even when the expression amount of FimE(wild-type) increases, the expression amount of GFP in the reporter cell (2) does not change. From this fact, we confirmed that the fim switch(wild-type) is inverted only from [ON] state to [OFF] state by FimE(wild-type). From the results of the two reporter cells (1) and (2), we successfully confirmed that FimE(wild-type) inverts the fim switch(wild-type) only from [ON] state to [OFF] state.
After measurement of flow cytometer, we minipreped the cell culture and got plasmid mixture which contain pSB6A1 and pSB3K3 in each sample.The state of fim switch(wild-type) either [ON] state or [OFF] state in colonies is evaluated from fluorescence. Thus, colonies which contain fim switch[default ON](wild-type) expressed GFP. On the other hand, colonies which contain fim switch[default OFF](wild-type) do not express GFP. We counted out the all colonies and those with fluorescence. In the results of the reporter cell (1), when inducing the expression of FimE(wild-type), the percentage of [ON] state decreased dramatically. On the other hand, from the results of the reporter cell (2), when inducing the expression of FimE(wild-type), the percentage of [ON] state remained being small. From the results of the two reporter cells (1) and (2), we successfully confirmed that FimE(wild-type) inverts the fim switch(wild-type) predominantly from [ON] state to [OFF] state. (Fig.6). This result was consistent with the histograms (Fig.5.).
Also, we incubated the colonies with fluorescence and those without fluorescence. We minipreped cell culture. Sequence complementarity in the specific region of the switch shows intended inversion of the switch from [ON] state to [OFF] state in all sample (Fig.7.).
More information
For more information, see http://2015.igem.org/Team:Tokyo_Tech/Project Our work in Tokyo_Tech 2015 wiki, http://2015.igem.org/Team:Tokyo_Tech/Experiment/ssrA_tag_degradation_assay About ssrA-tag, http://2015.igem.org/Team:Tokyo_Tech/Experiment/Overview_of_fim_inversion_system About ''fim'' inversion system
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000COMPATIBLE WITH RFC[1000]