Difference between revisions of "Part:BBa K731700"

 
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<partinfo>BBa_K731700 short</partinfo>
 
<partinfo>BBa_K731700 short</partinfo>
  
This part is used to analyse terminators: two subsequent fluorescent proteins (mCherry and A206K Venus), separated by Prefix-Suffix linker, allow standardization of terminator's presence effect. The vector is a modified pET21b; it contains Ampicillin resistance gene and is inducible by IPTG (T7promoter-lacO).
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Platform for terminators’ characterization by fluorimetric measurements and ratiometric analysis under IPTG inducible T7 promoter’s control  ([[Part:BBa_J64997|BBa_J64997]]).
 +
This backbone allows a precise and consistent measure of terminator’s effect on protein expression.
 +
It contains a bicistron of fluorescent proteins: mCherry first and then A206K Venus (mVenus). In between these two genes a BioBrick cloning region has been added, to insert the terminator to be tested. The comparison between the fluorescence of the two proteins with and without the terminator allows to derive some information about the terminator’s effect on protein expression.  
  
The combined use of [[Part:BBa_K731710|K731710]] and BBa_K731700 allow also to analyse any potential difference in terminators' activity due to different polymerases.
+
<div style="text-align:center">[[Image:K731700imageproject.jpg]]</div>
 +
 
 +
An almost identical backbone was also submitted as [[Part:BBa_K731710|BBa_K731710]]. To build it we used a type of insertion-deletion PCR to insert an ''E. coli tac'' transcriptional promoter and remove the T7 promoter. 
 +
The combined use of [[Part:BBa_K731710|BBa_K731710]] and BBa_K731700 allows also to analyze any potential difference in terminators' activity due to different RNA polymerases.
  
  
<!-- Add more about the biology of this part here
 
 
===Usage and Biology===
 
===Usage and Biology===
 +
We made some preliminary analyses to define the best procedure to use this platform.
 +
We found that the emission from mVenus was much stronger than the mCherry emission, resulting in some spectral overlap.  To improve the quality of the data, off-peak excitation and emission wavelengths were identified that minimized the effect. Therefore, mVenus was excitated at 485 nm (excitation peak is at 515 nm), and the emission of mVenus was collected at its maximum position, i.e. 528 nm.  The maximum mCherry excitation wavelength was used (587 nm), but the emission of mCherry was read at 615 nm, as opposed to the maximum at 610 nm.
 +
Here is a summary of these wavelengths:
 +
 +
 +
<div style="text-align:center">
 +
 +
{|border = "1" cellpadding="5" cellspacing="0" align="centre"
 +
|
 +
|Standard Excitation (nm)
 +
|Standard Emission (nm)
 +
|Modified Excitation (nm)
 +
|Modified Emission (nm)
 +
|-
 +
|mCherry
 +
|587
 +
|610
 +
|587
 +
|615
 +
|-
 +
|mVenus
 +
|515
 +
|528
 +
|485
 +
|528
 +
|}
 +
</div><html><p style="width:900px; text-align:justify "><em><strong>TABLE 1.</strong> <b>Standard and modified excitation and emission wavelengths. </b> We used these wavelengths for both in vivo and in vitro measurements.<br/></em> </p> </html>
 +
 +
 +
This part was used to characterize a T7 wild type terminator ([[Part:BBa_K731721|BBa_K731721]])and an ''E. coli'' terminator ([[Part:BBa_K731722|BBa_K731722]]).
 +
These terminators's activity was measured as the ratio between the two proteins'levels using the equation found in literature for termination efficiency.
 +
Doing this measurements, however, we realized that terminators can have an effect also on mCherry expression, enhancing it. This effect was previously described <cite>Abe</cite>. As a consequence of this unexpected outcome, we defined other two parameters that are here summarized in addition to the literature definition of termination efficiency:
 +
 +
The parameters used to analyze the data are:
 +
 +
apparent termination efficiency, calculated with the equation found in literature <cite>Nojima</cite>,    [[Image:FormulaEa.jpg]]
 +
 +
raw termination efficiency, that does not consider the mCherry contribution        [[Image:FormulaEr.jpg]]
 +
 +
relative increase in the upstream gene expression,      [[Image:RIequation.png]]
 +
 +
where
 +
 +
-''Vs'' is the A206K Venus peak’s intensity of the construct with the terminator of interest inserted in the prefix-suffix linker
 +
 +
-''Vc'' is the A206K Venus peak’s intensity of the control construct without intervening terminator
 +
 +
-''Cs'' is the mCherry peak’s intensity of the construct with the terminator inserted
 +
 +
-''Cc'' is the mCherry peak’s intensity of the control construct
 +
 +
 +
 +
''' ''In vivo'' measurements'''
 +
 +
Our experiments exploited an ''E. coli'' lysogen strain carrying T7 RNA polymerase and lacIq.  Additionally, the cells, i.e. ''E. coli'' BL21(DE3) pLysS, also contained a plasmid encoding T7 lysozyme and chloramphenicol resistance. T7 lysozyme is a natural inhibitor of T7 RNA polymerase activity, thus reducing background expression of the target genes.  The T7 RNA polymerase is behind a lacUV5 promoter.
 +
 +
 +
 +
<div style="text-align:center">[[Image:T7promoterinvivo.jpg]]</div>
 +
<p style="width:600px; margin-left:150px; margin-bottom:60px;
 +
text-align:justify "><em><strong>FIGURE 2.</strong> '''Results obtained from the ''in vivo'' measurements of [[Part:BBa_K731721|BBa_K731721]] (T7 terminator) and [[Part:BBa_K731722|BBa_K731722]] (''E. coli'' terminator) using BBa_K731700'''<br/>The data here analyzed were collected from cells that were expressed for 4 h with 0.1 mM isopropyl β-D-1-thiogalactopyranoside (IPTG).
 +
To identify optimal conditions, we screened samples that were and were not sonicated, sample dilutions to decrease the scattering of light, IPTG concentration, time of induction and time after induction.  We found that the best results were obtained with induction with 0.5 mM IPTG for 3 h, followed by sonication and centrifugation.  The cleared supernatant was then diluted 2-fold with phosphate buffer saline (PBS, 0.0067M PO4 without Ca or Mg, Cat number BE17-516F) and stored overnight at 4 °C.  Finally, fluorescence was measured with a Varian Cary Eclipse spectrofluorimeter using emission and excitation wavelengths described above, a slit of 5nm and a voltage of 570V.  The samples were left overnight at 4 °C to allow for sufficient time for the fluorescent proteins to properly mature (i.e. protein folding and chromophore formation).  Each measurement was made in quadruplicate from different colonies from different transformations and from different plates.
 +
</em> </p>
 +
 +
It is worth to highlight that the apparent and the raw transcriptional termination efficiencies, shown in figure 2, are essentially different from both a mathematical and a biological point of view. More specifically, raw termination efficiency is determined just by the expression of the downstream gene, while the apparent termination efficiency represents the variations that occur in the expression of both genes up- and down-stream of the terminator. They are in the same chart just for a comparison purpose.
 +
 +
For more information about the protocol we adopted to take these ''in vivo'' measurements, see [[BBa K731700 and BBa K731710 measurements]].
 +
 +
 +
'''''In vitro'' measurements'''
 +
 +
One potential reason for the increased mCherry levels could result from protection against cellular RNases.  Although RNases would not explain why the effect was only observed for the T7 terminator, we decided to test some of the constructs in a purified system that lacked the presence of nucleases.  Therefore, we exploited the PURExpress, which consists of purified transcription - translation machinery including T7 RNA polymerase and ''E. coli'' ribosomes. 
 +
 +
<div style="text-align:center">[[Image:K731700_invivovsinvitro1.jpg]]]</div>
 +
<p style="width:600px; margin-left:150px; margin-bottom:60px;
 +
text-align:justify "><em><strong>FIGURE 1.</strong> '''''[[Part:BBa_K731721|BBa_K731721]] T7 terminator's and [[Part:BBa_K731722|BBa_K731722]] ''E. coli'' terminator's transcriptional termination efficiencies'''<br/>The first chart shows the termination efficiencies as calculated in literature. The second graph represents the termination efficiencies calculated excluding the mCherry contribution. More specifically, the A206K Venus raw peaks were normalized over the control construct with no intervening terminator.
 +
 +
 +
</em> </p>
 +
 +
<div style="text-align:center">[[Image:K731700_mcherrygrowth_invivovsinvitro.jpg]]</div>
 +
 +
<div style="text-align:center">[[Image:K731700_mcherrygrowth_tab_invivovsinvitro.jpg]]</div>
 +
<p style="width:600px; margin-left:150px; margin-bottom:60px;
 +
text-align:justify "><em><strong>FIGURE 2.</strong> '''[[Part:BBa_K731721|BBa_K731721]] T7 terminator's and [[Part:BBa_K731722|BBa_K731722]] ''E. coli'' terminator's effects on mCherry expression'''<br/>This chart shows the raw emission peaks of mCherry normalized on the control construct without intervening terminator. Hence, the data can be interpreted as the time-folds of mCherry increase caused by the two terminators.
 +
 +
</em> </p>
 +
We submitted also this backbone with each terminator used in this study inserted in the cloning region as measurement plasmids; we hope that this could be helpful for anyone who want to verify and further delve into our results. They are [[Part:BBa_K731701|BBa_K731701]] for the T7 terminator and [[Part:BBa_K731702|BBa_K731702]] for the ''E. coli'' terminator.
 +
 +
More information about the procedure used, the results obtained and our considerations can be found in the  [http://2012.igem.org/Team:UNITN-Trento| Trento iGEM 2012 wiki page].
 +
 +
==References==
 +
<biblio>
 +
#Nojima pmid=16379390
 +
#Abe pmid=9150882
 +
</biblio>
 +
  
 
<!-- -->
 
<!-- -->

Latest revision as of 16:25, 11 October 2012

Platform for terminators analysis under the control of T7 promoter

Platform for terminators’ characterization by fluorimetric measurements and ratiometric analysis under IPTG inducible T7 promoter’s control (BBa_J64997). This backbone allows a precise and consistent measure of terminator’s effect on protein expression. It contains a bicistron of fluorescent proteins: mCherry first and then A206K Venus (mVenus). In between these two genes a BioBrick cloning region has been added, to insert the terminator to be tested. The comparison between the fluorescence of the two proteins with and without the terminator allows to derive some information about the terminator’s effect on protein expression.

K731700imageproject.jpg

An almost identical backbone was also submitted as BBa_K731710. To build it we used a type of insertion-deletion PCR to insert an E. coli tac transcriptional promoter and remove the T7 promoter. The combined use of BBa_K731710 and BBa_K731700 allows also to analyze any potential difference in terminators' activity due to different RNA polymerases.


Usage and Biology

We made some preliminary analyses to define the best procedure to use this platform. We found that the emission from mVenus was much stronger than the mCherry emission, resulting in some spectral overlap. To improve the quality of the data, off-peak excitation and emission wavelengths were identified that minimized the effect. Therefore, mVenus was excitated at 485 nm (excitation peak is at 515 nm), and the emission of mVenus was collected at its maximum position, i.e. 528 nm. The maximum mCherry excitation wavelength was used (587 nm), but the emission of mCherry was read at 615 nm, as opposed to the maximum at 610 nm. Here is a summary of these wavelengths:


Standard Excitation (nm) Standard Emission (nm) Modified Excitation (nm) Modified Emission (nm)
mCherry 587 610 587 615
mVenus 515 528 485 528

TABLE 1. Standard and modified excitation and emission wavelengths. We used these wavelengths for both in vivo and in vitro measurements.


This part was used to characterize a T7 wild type terminator (BBa_K731721)and an E. coli terminator (BBa_K731722). These terminators's activity was measured as the ratio between the two proteins'levels using the equation found in literature for termination efficiency. Doing this measurements, however, we realized that terminators can have an effect also on mCherry expression, enhancing it. This effect was previously described Abe. As a consequence of this unexpected outcome, we defined other two parameters that are here summarized in addition to the literature definition of termination efficiency:

The parameters used to analyze the data are:

apparent termination efficiency, calculated with the equation found in literature Nojima, FormulaEa.jpg

raw termination efficiency, that does not consider the mCherry contribution FormulaEr.jpg

relative increase in the upstream gene expression, RIequation.png

where

-Vs is the A206K Venus peak’s intensity of the construct with the terminator of interest inserted in the prefix-suffix linker

-Vc is the A206K Venus peak’s intensity of the control construct without intervening terminator

-Cs is the mCherry peak’s intensity of the construct with the terminator inserted

-Cc is the mCherry peak’s intensity of the control construct


In vivo measurements

Our experiments exploited an E. coli lysogen strain carrying T7 RNA polymerase and lacIq. Additionally, the cells, i.e. E. coli BL21(DE3) pLysS, also contained a plasmid encoding T7 lysozyme and chloramphenicol resistance. T7 lysozyme is a natural inhibitor of T7 RNA polymerase activity, thus reducing background expression of the target genes. The T7 RNA polymerase is behind a lacUV5 promoter.


T7promoterinvivo.jpg

FIGURE 2. Results obtained from the in vivo measurements of BBa_K731721 (T7 terminator) and BBa_K731722 (E. coli terminator) using BBa_K731700
The data here analyzed were collected from cells that were expressed for 4 h with 0.1 mM isopropyl β-D-1-thiogalactopyranoside (IPTG). To identify optimal conditions, we screened samples that were and were not sonicated, sample dilutions to decrease the scattering of light, IPTG concentration, time of induction and time after induction. We found that the best results were obtained with induction with 0.5 mM IPTG for 3 h, followed by sonication and centrifugation. The cleared supernatant was then diluted 2-fold with phosphate buffer saline (PBS, 0.0067M PO4 without Ca or Mg, Cat number BE17-516F) and stored overnight at 4 °C. Finally, fluorescence was measured with a Varian Cary Eclipse spectrofluorimeter using emission and excitation wavelengths described above, a slit of 5nm and a voltage of 570V. The samples were left overnight at 4 °C to allow for sufficient time for the fluorescent proteins to properly mature (i.e. protein folding and chromophore formation). Each measurement was made in quadruplicate from different colonies from different transformations and from different plates.

It is worth to highlight that the apparent and the raw transcriptional termination efficiencies, shown in figure 2, are essentially different from both a mathematical and a biological point of view. More specifically, raw termination efficiency is determined just by the expression of the downstream gene, while the apparent termination efficiency represents the variations that occur in the expression of both genes up- and down-stream of the terminator. They are in the same chart just for a comparison purpose.

For more information about the protocol we adopted to take these in vivo measurements, see BBa K731700 and BBa K731710 measurements.


In vitro measurements

One potential reason for the increased mCherry levels could result from protection against cellular RNases. Although RNases would not explain why the effect was only observed for the T7 terminator, we decided to test some of the constructs in a purified system that lacked the presence of nucleases. Therefore, we exploited the PURExpress, which consists of purified transcription - translation machinery including T7 RNA polymerase and E. coli ribosomes.

K731700 invivovsinvitro1.jpg]

FIGURE 1. BBa_K731721 T7 terminator's and BBa_K731722 E. coli terminator's transcriptional termination efficiencies
The first chart shows the termination efficiencies as calculated in literature. The second graph represents the termination efficiencies calculated excluding the mCherry contribution. More specifically, the A206K Venus raw peaks were normalized over the control construct with no intervening terminator.

K731700 mcherrygrowth invivovsinvitro.jpg
K731700 mcherrygrowth tab invivovsinvitro.jpg

FIGURE 2. BBa_K731721 T7 terminator's and BBa_K731722 E. coli terminator's effects on mCherry expression
This chart shows the raw emission peaks of mCherry normalized on the control construct without intervening terminator. Hence, the data can be interpreted as the time-folds of mCherry increase caused by the two terminators.

We submitted also this backbone with each terminator used in this study inserted in the cloning region as measurement plasmids; we hope that this could be helpful for anyone who want to verify and further delve into our results. They are BBa_K731701 for the T7 terminator and BBa_K731702 for the E. coli terminator.

More information about the procedure used, the results obtained and our considerations can be found in the [http://2012.igem.org/Team:UNITN-Trento| Trento iGEM 2012 wiki page].

References

<biblio>

  1. Nojima pmid=16379390
  2. Abe pmid=9150882

</biblio>


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Plasmid lacks a prefix.
    Plasmid lacks a suffix.
    Illegal EcoRI site found at 6850
    Illegal SpeI site found at 2
    Illegal PstI site found at 16
    Illegal NotI site found at 9
    Illegal NotI site found at 6856
  • 21
    INCOMPATIBLE WITH RFC[21]
    Plasmid lacks a prefix.
    Plasmid lacks a suffix.
    Illegal EcoRI site found at 6850
    Illegal BglII site found at 6011
    Illegal BamHI site found at 6832
    Illegal XhoI site found at 753
  • 23
    INCOMPATIBLE WITH RFC[23]
    Illegal prefix found at 6850
    Illegal suffix found at 2
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal prefix found at 6850
    Plasmid lacks a suffix.
    Illegal XbaI site found at 6865
    Illegal SpeI site found at 2
    Illegal PstI site found at 16
    Illegal NgoMIV site found at 714
    Illegal NgoMIV site found at 1051
    Illegal NgoMIV site found at 4231
    Illegal NgoMIV site found at 4391
    Illegal NgoMIV site found at 5979
    Illegal AgeI site found at 6800
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Plasmid lacks a prefix.
    Plasmid lacks a suffix.
    Illegal BsaI site found at 2228
    Illegal SapI.rc site found at 3310