Team:Northwestern/Results/Summary

From 2011.igem.org

Revision as of 03:23, 29 September 2011 by Rafay (Talk | contribs)

RETURN TO IGEM 2010



Overview


We characterized over two dozen parts over the course of this project. However, among the many, we will present the parts which represent our project best. These parts are [lasP+RBS30+GFP, CP+RBS30+lasR], [rhlP+RBS30+GFP, CP+RBS30+rhlR], and [GR(S)+RBS34+GFP, CP+RBS34+RhlR].


Binary Detection System


The construct [lasP+RBS30+GFP, CP+RBS30+lasR] is suited perfectly for conducting a binary test to determine the presence of P. Aeruginosa. Figure 1 below details the fluorescence per OD observed upon the induction of the system with multiple autoinducer concentrations. It is important to mention that there were 4 replicates of each autoinducer concentration sample, and the mean fluorescence per OD was plotted with the relevant error. In every case, the construct follows the same general trend except the negative control (0μM).


Figure 1: Fluorescence per OD for LasP+RBS30+GFP,CP+RBS30+lasR
fig1


There is significant amount of overlapping of error bars in the above Figure 1. In order to statistically confirm the variance of each concentration curve, t-tests were conducted as detailed below in Table 1. The null hypothesis is that there is no statistical difference between the means of the compared samples. On the other hand, the green cells indicate rejection of the null hypothesis that there is significant difference between the means of the compared samples. Blue cells indicate failure to reject. Table 1 has three sections: the top, center and bottom.


Table 1: Statistical testing table for lasP+RBS30+GFP, CP+RBS30+lasR. The null hypothesis is that there is no statistical difference between the means of the compared samples. Green cells indicate rejection of the null hypothesis, while blue cells indicate failure to reject.
fig1


The table on top compares the data from each of the initial segments of the curves with the other initial segments (the region before any fluorescence is observed ~30min). As the table indicates, most samples have no statistical difference than their counter parts, except of course for the 100μM which is induced quite quickly. Therefore we can conclude that the samples generally exhibit similar basal fluorescence.


The table in the middle compares the data from the initial segment of the curves (before any fluorescence is observed) with the final steady state fluorescence (last 10 data points). A glance at the table confirms that fluorescence per OD changes in each of the samples as time progresses. However, that seems to be the case with the negative control as well. Figure 1 demonstrates that the fluorescence per OD of the cell doesn’t increase, but decrease. This oddity is actually the result of steady fluorescence and a high rate of cell growth, which led to a sharp decrease in fluorescence per OD as shown in Figure 2 below.


Figure 2: Fluorescence and OD for lasP+RBS30+GFP, CP+RBS30+lasR
fig1


The table on the bottom compares the data from each of the final steady state segments of the curves with the other final steady state segments (last 10 data points). In this case, all the samples show no similar distributions of fluorescence except the 0.1μM, 0.5μM, and of course 0μM autoinducer concentrations. At first this may seem alarming, but it actually is not. In a binary test, simple detection is all that matters, whereas concentration sensitivity does not. When analyzing the steady state fluorescence and autoinducer concentration, one can observe that the fluorescence per OD is maintained fairly constant from within a 10% of the mean fluorescence per OD, illustrated by figure 3.


Figure 3: Fluorescence per OD vs. Autoinducer concentration for lasP+RBS30+GFP, CP+RBS30+lasR
fig1


Concentration Detection System


In contrast to the binary detection system, the construct [rhlP+RBS30+GFP, CP+RBS34+rhlR] is well suited for a conducting for determining the concentration of P. Aeruginosa by detecting and discriminating between various different concentrations of autoinducers. Figure 4 below details the fluorescence per OD observed upon the induction of the system with multiple autoinducer concentrations. Once again, there were 4 replicates of each autoinducer concentration sample, and the mean fluorescence per OD was plotted with the relevant error. Unlike the binary detection system, the fluorescence per OD of each of the curves is distinguishable from the other concentrations.


Figure 4: Fluorescence per OD for rhlP+RBS30+GFP, CP+RBS34+rhlR
fig1


For the most part, overlapping of error bars only occurs when the concentration of the autoinducer increases beyond 15μM which is not physiologically relevant. The resolution of the system can be demonstrated by figure 5, which clearly demonstrates that autoinducer concentrations between 0μM and 5μM are clear and distinguishable.


Figure 5: Fluorescence per OD for 0μM-5μM and 5μM-100μMrhlP+RBS30+GFP, CP+RBS34+rhlR
fig1


However, in order to statistically confirm the variance of each concentration curve, t-tests were conducted as detailed below in Table 2. The null hypothesis is that there is no statistical difference between the means of the compared samples. On the other hand, the green cells indicate rejection of the null hypothesis that there is significant difference between the means of the compared samples. Blue cells indicate failure to reject. Table 2 has three sections: the top, center and bottom.


Table 2: Statistical testing table for 0μM-5μM and 5μM-100μMrhlP+RBS30+GFP, CP+RBS34+rhlR. The null hypothesis is that there is no statistical difference between the means of the compared samples. Green cells indicate rejection of the null hypothesis, while blue cells indicate failure to reject.
fig1


The table on top compares the data from each of the initial segments of the curves with the other initial segments (the region before any fluorescence is observed ~30min). As one can observe, the samples predominantly are not statistically different than their counter parts, with except of course for the 100μM which is induced quite quickly, relative to the 0μM-5μM autoinducer samples. Hence it can be concluded that the samples exhibit similar basal fluorescence.


The table in the middle compares the data from the initial segment of the curves (before any fluorescence is observed) with the final steady state fluorescence (last 10 data points). Similar to the observation made in the binary system, each construct changes a statistically significant amount when exposed to the autoinducer. Unfortunately, so does the 0μM autoinducer sample. However, in this case, the induced constructs produce orders of magnitude more fluorescence than the negative control, so any cell bias introduced by either an OD irregularity is insignificant and can be ignored.


The table on the bottom compares the data from each of the final steady state segments of the curves with the other final steady state segments (last 10 data points). As can be observed, almost every single steady state fluorescence curve is different than the other. The two exceptions are the 7.5μM-10μM, and the 15μM-20μM autoinducer concentration samples. It is important to note that 10μM-15μM and 20μM-50μM concentration samples to indeed have statistically significant differences. In fact, the high degree of discrimination between relative autoinducer concentrations strongly qualifies this construct to be a concentration sensor. The steady state fluorescence per OD is conveyed in figure 6. The logarithmic regression fits the data quite well, and proves that the construct can potentially be used in as a sensor.


Figure 6: Fluorescence per OD vs. Autoinducer concentration for rhlP+RBS30+GFP, CP+RBS34+rhlR
fig1


Extracted Genomic Promoter Construct (Novel Entry)


In addition to designing plasmid systems using the existing and available biobricks, we also designed a plasmid containing an induced promoter extracted from the genome. Out of all the parts that we derived from the P. aeruginosa genome, the construct [GR(S)+RBS34+GFP, CP+RBS34+RhlR] was most suited to autoinducer detection. Figure 7 below details the fluorescence per OD observed upon the induction of the system with multiple autoinducer concentrations. In this case, the interval between successive data points is 7.5 minutes compared to the 5 minutes before. Additionally, the number of autoinducer concentrations tested for were less than in the previous characterizations; however, there were 4 replicates of each experimental sample.


Figure 7: Fluorescence per OD for GR(S)+RBS34+GFP, CP+RBS34+RhlR
fig1


Just as in the previous concentration detecting system, the genomic promoter system also discriminates very well between the varying autoinducer concentrations. To confirm our results, we conducted t-tests to validate the observed significance between the curves. The t-tests conducted follow the same format as the two described above and is detailed below in Table 3. The null hypothesis is that there is no statistical difference between the means of the compared samples. On the other hand, the green cells indicate rejection of the null hypothesis that there is significant difference between the means of the compared samples. Blue cells indicate failure to reject. Table 3 has three sections: the top, center and bottom.


Table 3: Statistical testing table for GR(S)+RBS34+GFP, CP+RBS34+RhlR. The null hypothesis is that there is no statistical difference between the means of the compared samples. Green cells indicate rejection of the null hypothesis, while blue cells indicate failure to reject.
fig1


The table on top compares the data from each of the initial segments of the curves with the other initial segments (the region before any fluorescence is observed ~30min). The statistical analysis of our novel genomic promoter construct turned out even better than that of our concentration detection system (discussed above). The initial data of almost every sample coincided with that of the negative control (0μM). Once again, the 100μM sample experienced induced fluorescence quite quickly. Thus, virtually all the samples exhibit fluorescence similar to that of the negative control.


The table in the middle compares the data from the initial segment of the curves (before any fluorescence is observed) with the final steady state fluorescence (last 10 data points). Similar to the observation made in the binary system, each construct changes a statistically significant amount when exposed to the autoinducer. The only outlying t-test in this characterization is the 0.1μM-20μM comparison, which may indicate that the uninduced state of the 20μM autoinducer sample was close to the induced state of the 0.1μM autoinducer sample’s fluorescence per OD. As the sole statistical irregularity it’s effect is insignificant.


The table on the bottom compares the data from each of the final steady state segments of the curves with the other final steady state segments (last 10 data points). Unquestionably, the data validates the claim that the fluorescence per OD of every single steady state curve is statistically different than the others. This result is further highlighted by the steady state fluorescence per OD vs. autoinducer concentration in figure 8. The low error and an extremely well fit logarithmic regression, and proves that the construct can not only works exactly the way it should, but is our most suited construct to be used in a sensor.


Figure 8: Fluorescence per OD vs. Autoinducer concentration for GR(S)+RBS34+GFP, CP+RBS34+RhlR
fig1


Model Fitting and Analysis


In the modelling section, the theoretical math behind the system was discussed. In order to fully understand our system, the mathematical model had to support the experimental data. Consequently, the sensitivity analysis was conducted (also in the modelling section) to gauge which factors influenced the system the most. A number of parameters were found to exert a significant amount of influence on the system. Each of these parameters was carefully adjusted until the theoretical graphs closely resembled those received from experimental testing as demonstrated below in figure 9.


Figure 9: Curve fit to the experimental data using the math model
fig1


Upon administration of the autoinducer concentration, the intracellular concentration of the autoinducer increases dramatically due to its passive transport through the cell membrane. Similarly, the initial concentration of R-protein is quite high relative to the other biochemical species in the cell due to its constitutive production. However, the increase in intracellular autoinducer concentration facilitates an instantaneous drop in the (free) R-protein concentration. The R-protein/dimer concentration level increases almost simultaneously, inducing the R-protein/autoinducer induced promoter. The sudden rise in the dimer complex facilitates a sudden increase in expression of the reporter construct or GFP. The concentration of GFP continually increases due to the increasing concentration of the dimer complex.


Autoinducer concentrations continue to drop until the reversible binding of the R-protein, autoinducer and the dimer complex reach steady state. This approximately happens at 150 minutes. At this point, most the autoinducer is bound to the dimer complex, and the remaining amount is degrading. In a way, the dimer complex is protecting the autoinducer from degradation, which maintains steady r-protein and dimer complex levels. Meanwhile GFP is being generated due to the initial excessive amount of reporter expression. However, when the R-protein and dimer complex reach steady state, so does GFP expression. additionally, the model fits the fluorescence data in the above characterization graphs. If one were to closely observe the GFP curve, the concentration actually decreases slightly over an extended period of time, which is exactly what was observed experimentally.


Conclusion


A brief overview of our analysis shows that our GFP constructs were extremely successful. Both the Las and Rhl reporter constructs exhibited fluorescence that was statistically significant relative to the controls at most or all of the autoinducer concentrations we tested. The Rhl promoters produced more fluorescence overall, but exhibited had a stronger concentration dependence (potentially indicating a broader dynamic range for these biosensors). The Las promoters produced very similar fluorescence values at almost every autoinducer concentration. These results provide an excellent characterization of the original registry promoters they are based on, as well as the constructs themselves. They also provide a solid basis for a device that can detect the presence of Pseudomonas Aeruginosa.


Our RFP constructs were not as successful. The results were inconsistent and the signals did not seem to be correlated to the presence of the autoinducersAlthough were not able to determine the cause of this problem, we have put the parts in the registry for future investigation.


In addition to working with the Las and Rhl dependent promoters already on the registry, we also characterized some new ones isolated directly from the Pseudomonas genome. This resulted in another potential set of promoters for use in a Pseudomonas detection device. In particular, the Rhl-dependent promoter we extracted showed excellent sensitivity to PAI2.


For complete characterization information on all of our parts, please refer to our Biobricks page. Clicking on a part will take you to the Registry of Standard Biological Parts, where the complete analysis for that part is posted.


Refer here for our testing protocol.



Sponsor northwestern.jpg Sponsor weinberg.jpg Sponsor mccormick.jpg