Team:Bielefeld-Germany/Project/Appoach

From 2012.igem.org

(Difference between revisions)
(Approach)
 
(68 intermediate revisions not shown)
Line 1: Line 1:
{{Team:Bielefeld/Head}}
{{Team:Bielefeld/Head}}
 +
<html>
 +
        <div id=page-title>
 +
            <span id=page-title-text>
 +
              Approach
 +
            </span>
 +
        </div>
 +
        <div id="grey_bg">
 +
</html>
 +
__TOC__
 +
<div style="text-align:justify;">
 +
The conventional methods of sewage treatment plants in order to take care of waste water are insufficient. This appears to be the case because most common microcontaminants like synthetic estrogen, bisphenol A, diclofenac ''etc.'' are very difficult to break down.
 +
The goal of Bielefeld's iGEM team is to develop a biological filter-system using immobilized laccases for the purification of municipal and industrial waste water to get rid of these synthetic estrogens and other aromatic compounds. Laccases are copper-containing oxidase enzymes found in many organisms. One of their properties is the ability to degrade a wide range of aromatic and phenolic compounds. For this purpose, genes of various bacterial and eukaryotic laccases were isolated and expressed in ''Escherichia coli'' and ''Pichia pastoris'' (see Fig. 1). The choice of the expression system was meanwhile dependent on the enzyme's glycosylation status.
-
<center>
+
[[File:File-Bielefeld2012_Approach_Isolation_Production_Purification.JPG|center|thumb|700px|'''Figure 1:''' The first steps of our project included the cloning, production and purification of the selected laccases from different organisms.]]
-
=Approach=
 
-
</center>
+
==Isolation of laccase genes and generation of new BioBricks==
-
The conventional methods in sewage treatment plants are unable to treat waste water sufficiently because the most frequently used micro contaminants like estrogen, Bisphenol A, Dicolfenac ''etc.'' are very difficult to break down.  
+
The first step of our project was to isolate the specific laccase gene sequences and to generate new BioBricks for the iGEM competition.
-
The goal of Bielefeld’s iGEM team is to develop a biological filtersystem using immobilized laccases to purify municipal and industrial wastewater from synthetic estrogens and other aromatic compounds. Laccases are copper-containing oxidase enzymes found in many organisms, and one of their properties is the ability to break down a wide range of aromatic and phenolic compounds. For this purpose, genes of various bacterial and eukaryotic laccases should be isolated and expressed in Escherichia coli and Pichia pastoris. The choice of the expressionsystem depends on the glycosylation status of the enzyme.
+
The laccases of the following organisms have been isolated:
-
==Isolation and Generating of new BioBricks==
+
'''Bacterial laccases from:'''
-
The first step for Step of our project is to isolate the specific gene sequences and to generate new BioBricks for the iGEM competition.
+
-
The Laccases of the following organisms are isolated:
+
-
'''bacterial laccases:'''[[File:Bielefeld2012_Approach_Isolation_Production_Purification.JPG|right|thumb|1200px|First steps of our Project]]
+
#''Escherichia coli''
 +
#''Bacillus halodurans''
 +
#''Bacillus pumilus''
 +
#''Streptomyces griseus''
 +
#''Streptomyces lavendulae''
 +
#''Thermus thermophilus''
 +
#''Xanthomonas campestris''
-
#Escherichia Coli
 
-
#Baccilus Halodurans
 
-
#Baccilus Pumilus
 
-
#Streptomyces griseus
 
-
#Streptomyces lavendulae
 
-
#Thermus thermophilus
 
-
#Xanthomonas campestris
 
 +
'''Eukaryotic laccases from:'''
-
''' Eukaryota laccases:'''
+
#''Arabidopsis thaliana''
 +
#''Pycnoporus cinnabarinus''
 +
#''Trametes versicolor''
 +
#''Trametes villosa''
-
#Arabidopsis thaliana
+
For more information about the organisms [https://2012.igem.org/Team:Bielefeld-Germany/Project/Background#4 click here].
-
#Tramestes versicolor
+
-
#Trametes villosa
+
-
 
+
The essential parts which were used to design our functional plasmids and a new shuttle-vector-system are listed in the following table:
-
For more information about the Organisms [[Team:Bielefeld-Germany/Project/Background/Organisms |click here]].
+
-
 
+
-
 
+
-
These BioBricks are used to design new plasmids and vector-systems. The diffenten parts to realise a functional Plasmid btw. Shuttle-Vector-System are shwon in the following table:
+
<center>
<center>
-
'''Parts of the ''E.coli'' Expressionvector and the ''P.Pastoris'' Shuttle-Vector'''
+
'''Parts of the ''E. coli'' expression vector and the ''P. pastoris'' shuttle vector'''
{|class="wikitable" style="text-align: center; width: 300px: height: 300px;" border=0}
{|class="wikitable" style="text-align: center; width: 300px: height: 300px;" border=0}
-
! Plasmid Characteristics  
+
! Plasmid characteristics  
-
! Shuttlevector Characteristics
+
! Shuttle vector characteristics
|-
|-
-
|T7 Promotorregion
+
|T7 promoter region
-
|AOX-Promotor
+
|AOX1 promoter
|-
|-
-
|His-Tag-Sequence
+
|His-Tag sequence
-
|alpha-factor
+
|Mating factor alpha 1
|-
|-
-
|Chloramphenicol Resistance
+
|Chloramphenicol resistance
-
|Zeocin Resistance
+
|Histidine auxotrophic complementation
|}
|}
Line 61: Line 67:
</center>
</center>
-
The Choice which expression system is used depends on the folding and glycosylation of the different laccases.   
+
The choice of the expression system was determined by the folding and glycosylation status of the individual laccase.   
-
The genetically modified organisms are used to produce different laccases.  Further down the line, these laccases are isolated and purified.
+
The resulting genetically modified organisms produced the laccases for our approach. In order to characterize the different laccases these enzymes have been isolated and purified.
 +
== Determining activity and potential of the different laccases ==
-
== Determining Activity and Potential of The Different Laccases ==
+
The next step to generate an efficient filter system was to characterize the purified laccases. To identify the potential of the laccases, each of the enzymes was examined for its activity and potential to degrade several substances. The degradation potential of the manufactured laccases was determined representatively for substances that originate from different chemical groups, such as analgesics, endocrine substances, pesticides, polycyclic aromatic hydrocarbons and bleaching agents (see Fig. 2).
 +
In our case, we analyzed the specific laccases for their degradation efficiency while varying different parameters like temperature, pH value and buffer system. A great concern of our team is to guarantee [https://2012.igem.org/Team:Bielefeld-Germany/Safety the safety] of the generated filter system. Besides the degradation potential, a very important aspect to us is the analysis of the degraded substances to ensure the harmlessness of the degradation result of an individual laccase. This was investigated and verified by HPLC-masspectroscopy (LC-ESI-qTOF-MS). With this knowledge, our aim was to identify the one laccase which shows the highest potential for a safe and highly functional filter system.
-
{|
+
[[File:Bielefeld2012_Substrates.png|center|thumb|450px|'''Figure 2:''' Representative substances from different chemical areas: endocrine substances (''estradiol, ethynyl estradiol, estrone''), pesticides (''lindane''), bleaching agent (''violuracid''), polycyclic aromatic hydrocarbons and analgesics (''diclofenac, naproxen, ibuprofen'')]]
-
|The next step to generate a effeciantally filter system is to characterize different produced and purified laccases. To identify the potential of different laccases, the enzyme are examined on their activity and the potential to degrade different substances. The degradation potential of different laccases are investigate for representative substances from different chemical areas like analgetics, endocrine substances, pesticides, poly aromatic hydrocarbons and bleaching agents.
+
== Immobilization and the final development of a degradation system==
-
In this case we analyses the efficiency of the laccase degradation and investigate different parameters like temperature, pH, and Buffer-systems. A great concern of our team is to guarantee the Safety of the generated filter system. Besides the degradation potential, a very important aspect is an analyzing of the degradated substances to guarantee, that the degradation with laccases don't generate any toxic or dangerous substances. These analyses realized by HPLC-massspectorscopy. With this knowledge we want to identify these laccase which show the highes potential for a functional filter system.
+
The last step for the realization of our project was to immobilize the produced laccase with the highest degradation potential. To generate a filter-system with a high yield of active and immobilized enzymes, different approaches were tested. On one hand, we tried to immobilize the enzymes with a chemical immobilization protocol to bind the laccases covalently on special silica-beads (CPC silica beads). On the other hand, we tried to generate an immobilization protocol by fusing the laccases to natural binding domains, such as the cellulose binding domain, the ceratin binding domain or the chitin binding domain. By establishing a new protocol, three different cellulose binding domains from the organisms ''Cellulomonas fimi'', ''Clostridium josui '' and ''Clostridium cellulovorans'' were investigated (see Fig. 3). In a first step, the binding-domains were linked to GFP (green fluorescent protein) in order to examine the strength of the binding and the binding-capacity. In the end, the domains will be fused to the laccases.
-
|[[File:Bielefeld2012_Substrates.png|right|thumb|450px|'''Representative substances''' from different chemical areas: Endocrine Substances (''Estradiol,Ethynylestradiol,Estrone''), Pesticides (''Lindane''), Bleaching Agent (''Violuracid''), Poly-Aromatic-Hydrocarbons and Analgetics(''Diclofenac, Naproxen, Ibuprofen'')]]  
+
[[File:Bielefeld2012_Immobilisierung_Approach.JPG|center|thumb|650px|'''Figure 3:''' Immobilization strategies]]
-
|}
+
-
== Immobilization and the final Development of the Filter==
+
The goal of the iGEM-Team Bielefeld was to generate a functional filter system with a high efficiency to degrade a high number of different microcontaminants. This filter system will be able to reduce the environmental pollution and improve the quality of waterbodies for the safety of animals and Mankind.
 +
</div>
 +
<html>
 +
  </div>
 +
</html>
-
The last step to realize our project is to immobilize the produced laccasses with the highes potentials. To generate a filtersystem with a high yield of active and immobilized enzymes different approaches are tested. One the one hand we try to immobilize the enzyme with a chemical immobilization protocol to bind covalent the laccases on specific silica-beads
+
{{Team:Bielefeld/Sponsoren}}

Latest revision as of 23:54, 2 December 2012

Approach

Contents

The conventional methods of sewage treatment plants in order to take care of waste water are insufficient. This appears to be the case because most common microcontaminants like synthetic estrogen, bisphenol A, diclofenac etc. are very difficult to break down. The goal of Bielefeld's iGEM team is to develop a biological filter-system using immobilized laccases for the purification of municipal and industrial waste water to get rid of these synthetic estrogens and other aromatic compounds. Laccases are copper-containing oxidase enzymes found in many organisms. One of their properties is the ability to degrade a wide range of aromatic and phenolic compounds. For this purpose, genes of various bacterial and eukaryotic laccases were isolated and expressed in Escherichia coli and Pichia pastoris (see Fig. 1). The choice of the expression system was meanwhile dependent on the enzyme's glycosylation status.

Figure 1: The first steps of our project included the cloning, production and purification of the selected laccases from different organisms.


Isolation of laccase genes and generation of new BioBricks

The first step of our project was to isolate the specific laccase gene sequences and to generate new BioBricks for the iGEM competition. The laccases of the following organisms have been isolated:

Bacterial laccases from:

  1. Escherichia coli
  2. Bacillus halodurans
  3. Bacillus pumilus
  4. Streptomyces griseus
  5. Streptomyces lavendulae
  6. Thermus thermophilus
  7. Xanthomonas campestris


Eukaryotic laccases from:

  1. Arabidopsis thaliana
  2. Pycnoporus cinnabarinus
  3. Trametes versicolor
  4. Trametes villosa

For more information about the organisms click here.

The essential parts which were used to design our functional plasmids and a new shuttle-vector-system are listed in the following table:

Parts of the E. coli expression vector and the P. pastoris shuttle vector

Plasmid characteristics Shuttle vector characteristics
T7 promoter region AOX1 promoter
His-Tag sequence Mating factor alpha 1
Chloramphenicol resistance Histidine auxotrophic complementation

The choice of the expression system was determined by the folding and glycosylation status of the individual laccase. The resulting genetically modified organisms produced the laccases for our approach. In order to characterize the different laccases these enzymes have been isolated and purified.


Determining activity and potential of the different laccases

The next step to generate an efficient filter system was to characterize the purified laccases. To identify the potential of the laccases, each of the enzymes was examined for its activity and potential to degrade several substances. The degradation potential of the manufactured laccases was determined representatively for substances that originate from different chemical groups, such as analgesics, endocrine substances, pesticides, polycyclic aromatic hydrocarbons and bleaching agents (see Fig. 2).

In our case, we analyzed the specific laccases for their degradation efficiency while varying different parameters like temperature, pH value and buffer system. A great concern of our team is to guarantee the safety of the generated filter system. Besides the degradation potential, a very important aspect to us is the analysis of the degraded substances to ensure the harmlessness of the degradation result of an individual laccase. This was investigated and verified by HPLC-masspectroscopy (LC-ESI-qTOF-MS). With this knowledge, our aim was to identify the one laccase which shows the highest potential for a safe and highly functional filter system.

Figure 2: Representative substances from different chemical areas: endocrine substances (estradiol, ethynyl estradiol, estrone), pesticides (lindane), bleaching agent (violuracid), polycyclic aromatic hydrocarbons and analgesics (diclofenac, naproxen, ibuprofen)

Immobilization and the final development of a degradation system

The last step for the realization of our project was to immobilize the produced laccase with the highest degradation potential. To generate a filter-system with a high yield of active and immobilized enzymes, different approaches were tested. On one hand, we tried to immobilize the enzymes with a chemical immobilization protocol to bind the laccases covalently on special silica-beads (CPC silica beads). On the other hand, we tried to generate an immobilization protocol by fusing the laccases to natural binding domains, such as the cellulose binding domain, the ceratin binding domain or the chitin binding domain. By establishing a new protocol, three different cellulose binding domains from the organisms Cellulomonas fimi, Clostridium josui and Clostridium cellulovorans were investigated (see Fig. 3). In a first step, the binding-domains were linked to GFP (green fluorescent protein) in order to examine the strength of the binding and the binding-capacity. In the end, the domains will be fused to the laccases.

Figure 3: Immobilization strategies

The goal of the iGEM-Team Bielefeld was to generate a functional filter system with a high efficiency to degrade a high number of different microcontaminants. This filter system will be able to reduce the environmental pollution and improve the quality of waterbodies for the safety of animals and Mankind.

55px Logo merck.jpg BioCircle.JPG Bielefeld2012 Evonik.jpg Bielefeld2012 Baxter.png Logo knauer.jpg Logo iit.jpg Bielefeld2012 BIEKUBA.jpg Logo biometra.jpg Logo bio-nrw.png Bielefeld2012 Logo ERASynbio.jpg