Difference between revisions of "Team:IIT-Madras/Model"

 
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__TOC__
  
  
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= Modularity of RBS parts =
<h2>Modularity of Ribosomal Binding Sites</h2>
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<p>Ribosomal Binding Site (RBS) part is the principle component in the translation process. It has been widely known that RBS parts are non-modular in nature and show variations in expression levels for different proteins. It has been argued that such variations are a combined result of thermal stability of mRNA molecules near RBS and codon bias.</p>
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<p>In regard to translation process, fundamental machinery in Prokaryotes and Eukaryotes are quite different. Transcription and translation processes are coupled in prokaryotes dissimilar to eukaryotes. This seems to be the probable cause of non-modular nature of RBS parts when they are used with different promoters to express the same protein, as we show at the end of this section.</p>
+
  
<p>In this section, we aim to provide a qualitative and quantitative information about the non-modular nature of RBS parts with respect to protein coding and promoter parts. We have used publicaly available expression data to validate an elementary model to predict the protein expression levels.</p>
+
== Introduction ==
 +
The '''non-modular nature''' of Ribosomal Binding Sites in bacteria is well known to the synthetic biology community. Most of the biological parts have been assigned a strength for their functionality. For example, Promoters have transcriptional score (number of RNA molecules per DNA molecule), RBSs have translational score (number of protein molecules per RNA molecule). Ideally, if we were to use a promoter and a RBS to produce a protein, we should get ('''transcriptional score times translational score''') number of protein molecules. In bacterial cells, transcription and translation processes are coupled and can occur simultaneously. This is why, these process are not independent and, hence, not modular. Apart from this, RNA molecules consisting of RBS and first few codons may form secondary structures, which in turn reduce the translation efficiency. Also, rare codons have also been shown to influence translation efficiency.
  
<p> <b>Note</b>: Apart from various researchers, previous year iGEM teams (2010 & 2011 Team Warsaw) have experimentally shown the non-modular nature of RBS parts.</p>
+
Secondary structure's and codons' influence on translational score of RBS are overlapping as they are a result of '''A, U, G, C''' combinations. Therefore, it is important to decouple both effects to unravel underlying patterns.
  
 +
'''We have successfully validated an empirical model to predict variations in protein expression levels, which could help future iGEM teams'''. Here, we represent a thorough description of our work.
  
<img src="https://static.igem.org/mediawiki/2016/f/fc/Iitmadras_model2_log2express.jpeg" width=800 height=470>
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== Methodology ==
  
<h2>Section 2</h2>
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The dataset from "Causes and effects of N-terminal codon bias in bacterial genes" paper was taken. Protein expression Data was available for following constructs :
<p>Content 2</p>
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2 promoters x 3 RBSs x 1781 (137x13) sfGFP variants in first 11 codons at N-terminal (3 RBS parts were B0034, B0032, B0030) and 2 promoter x 137 natural RBSs x 13 sfGFP variants in first 11 codons at N-terminal (2 Promoters were J23100 & J23108)
  
 +
== Hypothesis and Algorithm ==
 +
At the beginning, we hypothesized following things based on the information available in literature:<br>
 +
1. '''Expression is inversely proportional to the stability of secondary structure of mRNA near RBS part'''.<br>
 +
2. '''Rare codons present in first 11 codons of proteins have the ability to increase or decrease the translational score of RBS parts'''.<br>
 +
3. '''Each RBS part has a native strength irrespective of the promoter and protein coding part it can be used with'''.
  
 +
We designed an algorithm to compute the translational score of a given construct(which expresses a protein) in the following way:
 +
\begin{equation*}
 +
TS = \dfrac{NS*C_{pref}}{1+dG} + \alpha
 +
\end{equation*}
  
 +
\begin{equation*}
 +
C_{pref}= C_{1}*C_{2}*C_{3}*...*C_{11}*C_{sfGFP}
 +
\end{equation*}
  
</div>
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'''Objective Function''': minimize \(\sum \mid TS_{model}-TS_{experiment} \mid\)
  
</html>
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'''Outlier Removal''': top scores in \(\mid TS_{model}-TS_{experiment} \mid\)
 +
 
 +
where \(C_{i}\) is the codon preference of codon present at \(i^{th}\) position, \(C_{sfGFP}\) a constant for sfGFP protein codons, <br>
 +
'''TS''' : Translational Score of RBS part, <br>
 +
'''NS''' : Native Strength of RBS part,  which is equal to TS at \(\delta\)G=0, \(C_{pref}\)=1; <br>
 +
'''\(\delta\)G''' : Stability of RNA strand consisting of RBS and first 11 codon of protein, <br>
 +
\(\alpha\) is a constant.
 +
 
 +
== Quantification of Non-modularity ==
 +
As previously mentioned, RBS's have been found to be non-modular with respect to promoter and protein coding parts. A quantification of modularity would enable us to screen better RBS parts to make high order complex genetic circuits in high-throughput manner.
 +
 
 +
\begin{equation*}
 +
NM_p = \frac{\sigma_{NS}}{\langle {NS} \rangle} \\
 +
NM_c = \frac{\sigma_{TS}}{\langle {TS} \rangle}
 +
\end{equation*}
 +
where, '''NM<sub>p</sub>''' is non-modularity of RBS w.r.t. promoters; <br>
 +
'''NM<sub>c</sub>''' is non-modularity of RBS w.r.t. protein coding part; <br> '''NS''' is the array of native strength of RBS part with given promoters, <br> '''TS''' is the array of translational score of RBS part with given protein coding parts.
 +
 
 +
== Optimization ==
 +
Above model was optimized to compute the unknown variables, '''Native Strength of RBSs''' and '''codon preference matrix''', using the data from above mentioned paper. In MATLAB, <i>fmincon</i> function was used to minimize the sum of (\({TS_{model}-TS_{experiment})}^2\) for all 14137 constructs. After several iterations of optimization, we achieved following results. Optimization was done in MATLAB on a supercomputer facility at IIT Madras.
 +
Further, the system was optimized by removing 5%, 10% outliers, which were computed as the top scores in (\({TS_{model}-TS_{experiment})}^2\).
 +
 
 +
<gallery mode=nolines class=center widths=400px heights=230px caption="Validation of Model">
 +
File:Igemiitm_exp_model2.png|Experiment model, dark green 90% data, dark green+light dark green 95% data.
 +
File:Igemiitm_exp_model1.png|Null model, dark green 90% data, dark green+light dark green 95% data.
 +
</gallery>
 +
 
 +
 
 +
== Results ==
 +
<gallery class=center widths=400px heights=230px>
 +
File:Rbs_strength.png|Non-modularity of RBSs with Promoters
 +
File:Nonmodularity_of_B343230.png|Popular BioBrick RBS parts
 +
</gallery>
 +
 
 +
We found that some codons favor the translation process, while some of this do not. Following is a list of codons, which favor the translation process:
 +
 
 +
 
 +
{| class="wikitable" style="font-size:0.8em;@media screen and (max-width: 1000px){font-size:0.6em;}"
 +
! scope="row"| Codon
 +
|AAA||AAT||AGA||AGC||AGT||ATA||GAT||GGC||GGG||GGT||GTA||TCA||TCC||TCT||TGC
 +
|-
 +
! scope="row"| Amino Acid
 +
|K||N||R||S||S||I||D||G||G||G||V||S||S||S||C
 +
|-
 +
! scope="row"| Preference Value
 +
|1.17||1.23||1.15||1.13||1.21||1.14||1.13||1.19||1.19||1.21||1.14||1.14||1.13||1.19||1.19
 +
|-
 +
|}
 +
 
 +
Following is a list of codons, which reduces the translation efficiency:
 +
{| class="wikitable" style="font-size:0.8em;@media screen and (max-width: 1000px){font-size:0.6em;}"
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! scope="row"| Codon
 +
|CAC||CGC||CTC||GTC||TTC
 +
|-
 +
! scope="row"| Amino Acid
 +
|H||R||L||V||F
 +
|-
 +
! scope="row"| Preference Value
 +
|0.9768||0.9862||0.979||0.997||0.993
 +
|-
 +
|}
 +
 
 +
A complete list of codons and their preference values are [https://static.igem.org/mediawiki/2016/7/71/Igemiitm16_Codonpref.xlsx here]
 +
 
 +
 
 +
== Conclusion ==
 +
We could achieve a heuristic solution with a '''correlation of 0.87 with 90% of the data points''' for our experimental model, while null model gives us a correlation of 0.83 with 90% data points. Null model doesn't incorporate the feature of codon preference (C<sub>pref</sub>). As we see that codon preference feature improves our output, hence, it justifies the fact that codons can also vary translational score of RBS parts. Experimental model gives us the strength of promoter-RBS combined strength for 280 (2 promoters x 140 RBSs) combinations. This model provides a way to predict the variations in translational score of RBS parts unlike the existing tools. Using this model, users can get translational score for their expression systems.
 +
 
 +
= Noise in Devices =
 +
== Introduction ==
 +
In order to understand the behavior of device components, we need to have at least two signals coming from the device to understand the variations from '''intrinsic''' and '''extrinsic''' sources. Similarly, we can have two or more protein producing parts in complex biological devices, using which, we can understand the behavior of biological devices. [http://www.pnas.org/content/99/20/12795.short Elowtiz et al] has done significant work in understanding noise in biological devices. We have observed that if the mean value of one signal is bigger than the other signal, Elowitz formula doesn't give us accurate noise due to under-representation of variations present in low protein expressing device.
 +
 
 +
\begin{equation*}
 +
Noise_{int}=\frac{\langle {rfp-gfp} \rangle^2}{2*\langle gfp \rangle* \langle rfp \rangle};\\ 
 +
if \langle rfp \rangle > \langle gfp \rangle; Noise_{int} = \frac{{\langle rfp \rangle}^2}{2*\langle gfp \rangle*\langle rfp \rangle}; \\
 +
Noise_{int} = \frac{\langle {rfp} \rangle}{2*\langle gfp \rangle};
 +
\end{equation*}
 +
 
 +
<gallery class=center widths=400px heights=230px>
 +
File:Noise_var1.png|Signals from biological device
 +
</gallery>
 +
 
 +
== Solution ==
 +
To solve this problem, we have modified the current formula as follows:
 +
\begin{equation*}
 +
gr_{fold}=\dfrac{\langle rfp \rangle}{\langle gfp \rangle} \\
 +
Noise_{int}=\frac{\langle{rfp-gfp*gr_{fold}}\rangle^2}{2*\langle gfp \rangle*\langle rfp \rangle*gr_{fold}};\\ 
 +
\end{equation*}
 +
 
 +
<gallery class=center widths=400px heights=230px center>
 +
File:Noise_var2.png|Corrected Signals from biological device
 +
</gallery>
 +
 
 +
== References ==
 +
[http://science.sciencemag.org/content/342/6157/475 1.] Goodman, Daniel B., George M. Church, and Sriram Kosuri. "Causes and effects of N-terminal codon bias in bacterial genes." Science 342.6157 (2013): 475-479.
 +
{{IIT-Madras-Bottom/CSS}}

Latest revision as of 23:40, 19 October 2016


Modularity of RBS parts

Introduction

The non-modular nature of Ribosomal Binding Sites in bacteria is well known to the synthetic biology community. Most of the biological parts have been assigned a strength for their functionality. For example, Promoters have transcriptional score (number of RNA molecules per DNA molecule), RBSs have translational score (number of protein molecules per RNA molecule). Ideally, if we were to use a promoter and a RBS to produce a protein, we should get (transcriptional score times translational score) number of protein molecules. In bacterial cells, transcription and translation processes are coupled and can occur simultaneously. This is why, these process are not independent and, hence, not modular. Apart from this, RNA molecules consisting of RBS and first few codons may form secondary structures, which in turn reduce the translation efficiency. Also, rare codons have also been shown to influence translation efficiency.

Secondary structure's and codons' influence on translational score of RBS are overlapping as they are a result of A, U, G, C combinations. Therefore, it is important to decouple both effects to unravel underlying patterns.

We have successfully validated an empirical model to predict variations in protein expression levels, which could help future iGEM teams. Here, we represent a thorough description of our work.

Methodology

The dataset from "Causes and effects of N-terminal codon bias in bacterial genes" paper was taken. Protein expression Data was available for following constructs : 2 promoters x 3 RBSs x 1781 (137x13) sfGFP variants in first 11 codons at N-terminal (3 RBS parts were B0034, B0032, B0030) and 2 promoter x 137 natural RBSs x 13 sfGFP variants in first 11 codons at N-terminal (2 Promoters were J23100 & J23108)

Hypothesis and Algorithm

At the beginning, we hypothesized following things based on the information available in literature:
1. Expression is inversely proportional to the stability of secondary structure of mRNA near RBS part.
2. Rare codons present in first 11 codons of proteins have the ability to increase or decrease the translational score of RBS parts.
3. Each RBS part has a native strength irrespective of the promoter and protein coding part it can be used with.

We designed an algorithm to compute the translational score of a given construct(which expresses a protein) in the following way: \begin{equation*} TS = \dfrac{NS*C_{pref}}{1+dG} + \alpha \end{equation*}

\begin{equation*} C_{pref}= C_{1}*C_{2}*C_{3}*...*C_{11}*C_{sfGFP} \end{equation*}

Objective Function: minimize \(\sum \mid TS_{model}-TS_{experiment} \mid\)

Outlier Removal: top scores in \(\mid TS_{model}-TS_{experiment} \mid\)

where \(C_{i}\) is the codon preference of codon present at \(i^{th}\) position, \(C_{sfGFP}\) a constant for sfGFP protein codons,
TS : Translational Score of RBS part,
NS : Native Strength of RBS part, which is equal to TS at \(\delta\)G=0, \(C_{pref}\)=1;
\(\delta\)G : Stability of RNA strand consisting of RBS and first 11 codon of protein,
\(\alpha\) is a constant.

Quantification of Non-modularity

As previously mentioned, RBS's have been found to be non-modular with respect to promoter and protein coding parts. A quantification of modularity would enable us to screen better RBS parts to make high order complex genetic circuits in high-throughput manner.

\begin{equation*} NM_p = \frac{\sigma_{NS}}{\langle {NS} \rangle} \\ NM_c = \frac{\sigma_{TS}}{\langle {TS} \rangle} \end{equation*} where, NMp is non-modularity of RBS w.r.t. promoters;
NMc is non-modularity of RBS w.r.t. protein coding part;
NS is the array of native strength of RBS part with given promoters,
TS is the array of translational score of RBS part with given protein coding parts.

Optimization

Above model was optimized to compute the unknown variables, Native Strength of RBSs and codon preference matrix, using the data from above mentioned paper. In MATLAB, fmincon function was used to minimize the sum of (\({TS_{model}-TS_{experiment})}^2\) for all 14137 constructs. After several iterations of optimization, we achieved following results. Optimization was done in MATLAB on a supercomputer facility at IIT Madras. Further, the system was optimized by removing 5%, 10% outliers, which were computed as the top scores in (\({TS_{model}-TS_{experiment})}^2\).


Results

We found that some codons favor the translation process, while some of this do not. Following is a list of codons, which favor the translation process:


Codon AAA AAT AGA AGC AGT ATA GAT GGC GGG GGT GTA TCA TCC TCT TGC
Amino Acid K N R S S I D G G G V S S S C
Preference Value 1.17 1.23 1.15 1.13 1.21 1.14 1.13 1.19 1.19 1.21 1.14 1.14 1.13 1.19 1.19

Following is a list of codons, which reduces the translation efficiency:

Codon CAC CGC CTC GTC TTC
Amino Acid H R L V F
Preference Value 0.9768 0.9862 0.979 0.997 0.993

A complete list of codons and their preference values are here


Conclusion

We could achieve a heuristic solution with a correlation of 0.87 with 90% of the data points for our experimental model, while null model gives us a correlation of 0.83 with 90% data points. Null model doesn't incorporate the feature of codon preference (Cpref). As we see that codon preference feature improves our output, hence, it justifies the fact that codons can also vary translational score of RBS parts. Experimental model gives us the strength of promoter-RBS combined strength for 280 (2 promoters x 140 RBSs) combinations. This model provides a way to predict the variations in translational score of RBS parts unlike the existing tools. Using this model, users can get translational score for their expression systems.

Noise in Devices

Introduction

In order to understand the behavior of device components, we need to have at least two signals coming from the device to understand the variations from intrinsic and extrinsic sources. Similarly, we can have two or more protein producing parts in complex biological devices, using which, we can understand the behavior of biological devices. [http://www.pnas.org/content/99/20/12795.short Elowtiz et al] has done significant work in understanding noise in biological devices. We have observed that if the mean value of one signal is bigger than the other signal, Elowitz formula doesn't give us accurate noise due to under-representation of variations present in low protein expressing device.

\begin{equation*} Noise_{int}=\frac{\langle {rfp-gfp} \rangle^2}{2*\langle gfp \rangle* \langle rfp \rangle};\\ if \langle rfp \rangle > \langle gfp \rangle; Noise_{int} = \frac{{\langle rfp \rangle}^2}{2*\langle gfp \rangle*\langle rfp \rangle}; \\ Noise_{int} = \frac{\langle {rfp} \rangle}{2*\langle gfp \rangle}; \end{equation*}

Solution

To solve this problem, we have modified the current formula as follows: \begin{equation*} gr_{fold}=\dfrac{\langle rfp \rangle}{\langle gfp \rangle} \\ Noise_{int}=\frac{\langle{rfp-gfp*gr_{fold}}\rangle^2}{2*\langle gfp \rangle*\langle rfp \rangle*gr_{fold}};\\ \end{equation*}

References

[http://science.sciencemag.org/content/342/6157/475 1.] Goodman, Daniel B., George M. Church, and Sriram Kosuri. "Causes and effects of N-terminal codon bias in bacterial genes." Science 342.6157 (2013): 475-479.