IGEM:IMPERIAL/2007/Experimental Design/Phase1/Results 1.1: Difference between revisions

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=Results summary=
= ''In vivo'' Testing of pTet-GFP and pT7-GFP Constructs=
<br><br>


===[http://parts.mit.edu/registry/index.php/Part:BBa_I13522 '''pTet-GFP'''] ===
__NOTOC__
<br>
==Aims==
The pTet - GFP construct has been successfully tested in vivo. The levels of fluorescence of the construct where comparable to the levels of our positive control (200x dilution of GFP) meaning that GFP was actually produced. Therefore pTet-GFP works in E.Coli.
To determine if the following constructs work in vivo:
<br><br>
*[http://parts.mit.edu/registry/index.php/Part:BBa_I13522 '''pTet-GFP''']  
*[http://parts.mit.edu/registry/index.php/Part:BBa_E7104 '''pT7-GFP''']


The testing was comprised of several tests:
*pTet and pT7 ''in vivo'' - [[IGEM:IMPERIAL/2007/Notebook/2007-8-16 | Tested 15-08-2007]]
*Retesting pT7 ''in vivo'' - [[IGEM:IMPERIAL/2007/Notebook/2007-8-17 | Tested 17-08-2007]]


* A 1 hour run (taking measurements every 2.5 min) was also conducted to test the variation on the expression levels of pTet-GFP over time.
== Materials and Methods ==
<br><br>
Refer to protocols page.
[[Image:IC2007 Experiments Phase1 Protocol1-1Res.jpg |thumb|left|400px| Results of testing pTet and pT7 at 0.15 sec counting time for fluorometer detector]]


[[Image:IC2007 Experiments Phase1 Protocol1-1.jpg |thumb|none|560px| Results of testing pTet and pT7 at 0.15 sec counting time for fluorometer detector]]


==Results==
====<font color=darkblue>''Test: 17-08-2007''</font>====
{|align="left"
| width="200px"|[[Image:IC2007 Experiments Phase1 Protocol1-1Res.JPG|thumb|300px|Fig.1: Total Fluorescence of pTet-GFP and pT7-GFP ''in vivo'' over 6 hours]]
| width="200px"| [[Image:IC2007 Experiments Phase1 Protocol1-1.jpg|thumb|300px|Fig.2: pTet ''in vivo'' over 6 hours]]
| width="50px"|
|width="300px"| pTet-GFP and pT7-GFP were both compared to a negative and positive control, where pTet-GFP showed significant fluorescence, while pT7 did not show any dramatic increase (Fig.1). When measured over intervals, pTet showed a steady increase in fluorescence (Fig.2). Fig.2 also suggests that there may be some variation across the samples that have been measured.
|}
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====<font color=darkblue>''Test: 21-08-2007</font>''====
{|align="left"
| width="200px"| [[Image:IC2007 Experimental design protocol1-1res2 .PNG|thumb|280px| Fig.3 - Total Fluorescence of pT7-GFP ''in vivo'' over 4 hours]]
| width="200px"| [[Image:IC2007 Experiments Phase1 Protocol1-1Res1.PNG|thumb|310px|Fig.4 - pT7-GFP ''in vivo'' over 4 hours]]
| width="50px"|
|width="300px"| Fig.3 shows that the pT7-GFP construct had significant fluorescence compared to the negative control, which seems to suggest that GFP has been expressed. However, when fluorescence correlated over the time period, there was little or no increase in fluorescence (Fig.4), suggesting little or no expression of GFP over the time course.
|}
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<br clear="all">


<br><br>
'''Controls:'''
 
*Positive control - diluted GFP solution of equal volume
===[http://parts.mit.edu/registry/index.php/Part:BBa_E7104 '''pT7-GFP''']===
*Negative control - LB media of equal volume
<br>
Initial testing of the pT7 - GFP contruct in vivo failed because it was not properly induced. It will be re-tested on the 17/08/2007 after it has been induced with IPTG and left overnight to allow for a measurable GFP amount to be produced. IPTG is a T7 inducer for the E.Coli strain used (BL21).
<br>
 
====Results update: 17/8/2007====
After re-testing the pT7-GFP in vivo, no positive fluorescence reading was observed. The fluorescence levels were recorded over a range of 4 hours for 3 repeats and compared, as in the case of pTet, to a positive control of diluted GFP. The temperature used throughout the experiments was room temperature (thermometer reading at 25oC).
 
[[Image:IC2007 Experiments Phase1 Protocol1-1Res1.PNG |thumb|left|500px| Results of in vivo testing of pT7 over a 4 hour period ]]
 
<br><br>
On the graph on the right we see the averaged-out fluorescence of the 3 repeats of the pT7-GFP assembly, compared to the diluted GFP solution used as a positive control. The fluorescence activity of pT7-GFP is minimal and remains at a constant basal level. This allows us to conclude that the pT7-GFP contruct does not work as fast as pTet in vivo or it does not work at all. Two reasons were hypothesized:


1). The bacteria cells were in stationary phase <br>
[http://openwetware.org/images/4/42/IC2007_Experiments_Phase_1_Results-16-08-2007.xls  Complete set of results and raw data ]
2). The pT7 construct is not working.


<br><br>
A second test will be performed to test whether the low readings were due to extremely slow activation of the pT7 promoter or the inefficiency of the construct.
<br clear="all">
<br clear="all">
<br>


====Results update: 21/8/2007====
==Discussion==
===[http://parts.mit.edu/registry/index.php/Part:BBa_I13522 '''pTet-GFP''']===
Fig.1 and Fig.2 both strongly indicate that there was a good amount of expression of GFP (~54000) with the pTet-GFP construct, leading to an increase in fluoresence over time. This shows that the construct is functioning well ''in vivo''.


A second in vivo test of the pT7-GFP contruct has been performed to test if the construct actually works. The pT7-GFP was induced with iPTG and left overnight at a temperature of ???? . Three repeats were carried out to verify our results. The fluorescence reading was taken at the start of the experiment (21/8/2007 10:00 AM)  , 7 hours later (21/8/2007 05:00 PM) and 24 hours later (22/08/2007 10:00 AM).
Fig.2 however suggests that there may be significant variation in the measurement of our samples. This could be due to experimental methodology, or the intrinsic nature of variability of expression in the ''in vivo'' chassis.


[[Image:IC2007 Experimental design protocol1-1res2 .PNG |thumb|left|500px| Results of in vivo testing of pT7 over a 24 hour period ]]


<br><br> From the graph on the right, we can conclude that pT7-GFP is not functioning properly. The graph shows the averaged out value of fluorescence reading of the 3 samples of pT7-GFP used as reapeats. Minute amounts of fluorescence have been recorded but it is 5 times less than the results recorded with pTet-GFP. It is now safe to conclude that the pT7-GFP assembly is not working in vivo. Further tests will be carried out in vitro as planned in a hope that using that chassis we will get better results.
===[http://parts.mit.edu/registry/index.php/Part:BBa_E7104 '''pT7-GFP''']===
 
As our initial tests of the pT7-GFP construct did not yield expected results, it was postualated that the absence of fluorescence increase could be due to several reasons. Firstly, the cells might not be properly induced, to which IPTG of a suitable concentration(~1mM) needs to be added, and the culture grown overnight. It could also be that the construct was not working at all, or that the culture was in stationary phase when it was tested, leading to little or not expression of GFP.
<br clear="all">


===[http://parts.mit.edu/registry/index.php/Part:BBa_I719022 '''pCI-GFP''']===
In the re-test, the culture had been properly induced with IPTG at growth phase. While absolute fluorescence levels indicate the presence of GFP in the culture, it was not as significant as that of pTet-GFP. In addition, there was little or no increase of fluorescence over the time period at which it was measured. This could be due to the fact that the pT7-GFP construct either did not express as quickly or strongly as pTet-GFP ''in vivo'', or that the construct was simply not working. Further investigation into the construct also revealed a weaker ribosome binding site compared to the pTet-GFP construct which could account for the weak fluorescent signal.  
Testing of the assembly has been postponed due to delays in the making of the construct. Testing will be carried out as soon as the construct is ready.
<br>


====Results update: 21/8/2007====
After numerous attempts to grow the pCI-GFP construct, it is found to be unavailable in the respository sent by the MIT and hence cannnot be grown and implemented in our experiments. Testing of this construct has been abandoned.


 
==Conclusion==
{| border="2" style="background:#ABCDEF;" align=center
We investigated the possibility of using different constructs, and strength of different promoters for our projects. To conclude,
| [http://openwetware.org/images/4/42/IC2007_Experiments_Phase_1_Results-16-08-2007.xls  Complete set of results and raw data ].
* pTet-GFP construct gave a strong fluorescent signal, indicating good expression of GFP ''in vivo''.
|}
* pT7-GFP construct gave little or no fluorescent signal, to which several reasons had been suggested, and further experiments are required to corrobate them.

Latest revision as of 05:26, 14 October 2007

In vivo Testing of pTet-GFP and pT7-GFP Constructs

Aims

To determine if the following constructs work in vivo:

The testing was comprised of several tests:

Materials and Methods

Refer to protocols page.


Results

Test: 17-08-2007

Fig.1: Total Fluorescence of pTet-GFP and pT7-GFP in vivo over 6 hours
Fig.2: pTet in vivo over 6 hours
 pTet-GFP and pT7-GFP were both compared to a negative and positive control, where pTet-GFP showed significant fluorescence, while pT7 did not show any dramatic increase (Fig.1). When measured over intervals, pTet showed a steady increase in fluorescence (Fig.2). Fig.2 also suggests that there may be some variation across the samples that have been measured.


Test: 21-08-2007

Fig.3 - Total Fluorescence of pT7-GFP in vivo over 4 hours
Fig.4 - pT7-GFP in vivo over 4 hours
 Fig.3 shows that the pT7-GFP construct had significant fluorescence compared to the negative control, which seems to suggest that GFP has been expressed. However, when fluorescence correlated over the time period, there was little or no increase in fluorescence (Fig.4), suggesting little or no expression of GFP over the time course.


Controls:

  • Positive control - diluted GFP solution of equal volume
  • Negative control - LB media of equal volume

Complete set of results and raw data


Discussion

pTet-GFP

Fig.1 and Fig.2 both strongly indicate that there was a good amount of expression of GFP (~54000) with the pTet-GFP construct, leading to an increase in fluoresence over time. This shows that the construct is functioning well in vivo.

Fig.2 however suggests that there may be significant variation in the measurement of our samples. This could be due to experimental methodology, or the intrinsic nature of variability of expression in the in vivo chassis.


pT7-GFP

As our initial tests of the pT7-GFP construct did not yield expected results, it was postualated that the absence of fluorescence increase could be due to several reasons. Firstly, the cells might not be properly induced, to which IPTG of a suitable concentration(~1mM) needs to be added, and the culture grown overnight. It could also be that the construct was not working at all, or that the culture was in stationary phase when it was tested, leading to little or not expression of GFP.

In the re-test, the culture had been properly induced with IPTG at growth phase. While absolute fluorescence levels indicate the presence of GFP in the culture, it was not as significant as that of pTet-GFP. In addition, there was little or no increase of fluorescence over the time period at which it was measured. This could be due to the fact that the pT7-GFP construct either did not express as quickly or strongly as pTet-GFP in vivo, or that the construct was simply not working. Further investigation into the construct also revealed a weaker ribosome binding site compared to the pTet-GFP construct which could account for the weak fluorescent signal.


Conclusion

We investigated the possibility of using different constructs, and strength of different promoters for our projects. To conclude,

  • pTet-GFP construct gave a strong fluorescent signal, indicating good expression of GFP in vivo.
  • pT7-GFP construct gave little or no fluorescent signal, to which several reasons had been suggested, and further experiments are required to corrobate them.
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