Difference between revisions of "Team:Freiburg/Results/Immobilization"

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Coupling of DNA to the PDMS slide was achieved using a DNA concentration of 25&nbsp;ng/µl. Either 1 or 3 µl of DNA were spotted directly onto the slide using a distinct pattern (figure 2A). To verify that only the amino-labeled DNA binds specifically, we added spots of non-amino-labeled DNA as a negative control. The slide was subsequently incubated over night and the DNA solution was washed away with ddH<sub>2</sub>O. After drying, examination of the PDMS flow cell by fluorescence microscopy showed the pattern illustrated in figure 2B. The resulting fluorescence pattern clearly corresponds to the spotting pattern on the slide, thereby confirming that the immobilization of DNA was successful. Spots that were incubated with amino-labeled DNA show a distinct Cy3 fluorescence signal, whereas DNA that was not labeled with an amino group had not bound to the surface.  
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Coupling of DNA to the PDMS slide was achieved using a DNA concentration of 25&nbsp;ng/µl. Either 1 or 3 µl of DNA were spotted directly onto the slide using a distinct pattern (figure 2A). To verify that only the amino-labeled DNA binds specifically, we added spots of non-amino-labeled DNA as a negative control. The slide was subsequently incubated over night and the DNA solution was washed away with ddH<sub>2</sub>O. After drying, examination of the PDMS flow cell at 532 nm by fluorescence microscopy showed the pattern illustrated in figure 2B. The resulting fluorescence pattern clearly corresponds to the spotting pattern on the slide, thereby confirming that the immobilization of DNA was successful. Spots that were incubated with amino-labeled DNA show a distinct Cy3 fluorescence signal, whereas DNA that was not labeled with an amino group had not bound to the surface.  
 
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<h2>Cell-Free Expression of GFP From Spotted DNA</h2>
 
  
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<h2>Cell-Free Expression of GFP From DNA Spots</h2>
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                       <p><strong>Figure 3: GFP expressed from immobilized DNA.</strong> Fluorescence microscopy was used to visualize GFP after expression of immobilized DNA. Expression was performed for 2 h using our DiaMIX and immobilization of the His-tagged GFP was obtained by our Ni-NTA surface.</p>
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                       <p><strong>Figure 3: Fluorescent GFP spots after 30 min of cell-free expression.</strong> The fluorescence was measured by placing the assembled chamber under a microscope. The system still was filled with expression mix.</p>
 
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In addition to DNA immobilization itself, it is important to show that the immobilized sequence is still capable of being transcribed and translated. Therefore, the sequence was designed to contain all important elements for protein expression as promoter, ribosomal binding site and terminator. Additionally, it was adapted to the requirements of a cell-free expression system.  
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Having verified that DNA can be bound to the PDMS flow cell, the next step was showing that the immobilized sequence is still capable of being transcribed and translated.
 
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The microfluidic chamber consisting of the PDMS slide and an activated glass slide was assembled after immobilization of a GFP expression cassette. Using the microfluidic system, the DiaCHIP was flushed with our DiaMIX enabling cell-free expression to take place. To achieve a high yield of expressed GFP, the expression was performed for 2 h at room temperature. The glass slide was covered with our specific Ni-NTA surface. Thus, only His-tagged GFP is immobilized on the opposite site of the chamber, while other components of the DiaMIX are washed away after the expression.
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The microfluidic chamber consisting of the PDMS slide and a glass slide with a specific Ni-NTA surface was then assembled and filled with cell-free expression mix. The expression was performed for 2 h at 37°C.  
 
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The glass slide was analyzed by fluorescence microscopy afterwards. As it is shown in figure 3, cell-free expressed GFP was imobilized in distinct spots and exhibited a fluorescence signal. Thus, besides being expressed, the protein was also correctly folded and remains functional.  
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The microfluidic chamber was analyzed by fluorescence microscopy afterwards. As shown in figure 3, cell-free expressed GFP was observed in distinct spots exhibiting a clear fluorescence signal. Thus, besides being expressed, the protein was also correctly folded and remained functional.
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Revision as of 19:44, 18 September 2015

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Cell-Free Expression of Immobilized DNA

An important advantage of the DiaCHIP is the possibility to ship and store information encoded by DNA. From a DNA template array protein arrays can be produced on demand. In order to obtain this template, DNA is fixed on a silicone slide forming one side of our microfluidic chamber. Making use of a cell-free expression system, the DNA can then be transcribed and translated into the respective proteins resulting in the final protein array. The coding sequence of the proteins is genetically fused to a tag allowing their binding to a specific surface on the opposite side of the chamber.

Successful binding of DNA to the Silicone Slide

Figure 1: Scheme of the APTES/PDITC surface. The PDMS (red) is layered with APTES (light grey) and the amino-linker PDITC (dark grey). The hydroxy layer generated during plasma activation is represented in blue.

The core component of the DiaCHIP is the microfluidic chamber composed of a glass slide for protein immobilization and a PDMS (polydimethylsiloxane) flow cell. The silicone PDMS needs to be activated to enable the generation of the DNA template array by binding of the respective sequences. Oxygen plasma is used to initially activate the surface of the PDMS slide by generating a hydroxy layer. This allows linking the silane APTES and finally the crosslinker PDITC. In order to bind the DNA covalently to this surface the respective DNA sequence requires an N- or C-terminal amino group. The structure of this surface is schematically visualized in figure 1. This surface chemistry is identical to the protocol used to immobilize proteins on a glass slide unspecifically (see PDITC surface for immobilizing proteins).
In order to obtain an expression cassette for GFP with an amino group, the target sequence was amplified by PCR using an amino-labeled reverse primer. Additionally, the forward primer was labeled by the fluorescent dye Cy3 to enable visualization by fluorescence microscopy. Successful amplification of the target sequence was verified by agarose gel electrophoresis.

Figure 2: Immobilization of DNA on a PDMS slide. A: Top view on the slide indicating the spotting pattern. B: Cy3 fluorescence showing successful immobilization of amino-labeled DNA. As a negative control, Cy3-labeled DNA without amino group was spotted (indicated by white circles).

Coupling of DNA to the PDMS slide was achieved using a DNA concentration of 25 ng/µl. Either 1 or 3 µl of DNA were spotted directly onto the slide using a distinct pattern (figure 2A). To verify that only the amino-labeled DNA binds specifically, we added spots of non-amino-labeled DNA as a negative control. The slide was subsequently incubated over night and the DNA solution was washed away with ddH2O. After drying, examination of the PDMS flow cell at 532 nm by fluorescence microscopy showed the pattern illustrated in figure 2B. The resulting fluorescence pattern clearly corresponds to the spotting pattern on the slide, thereby confirming that the immobilization of DNA was successful. Spots that were incubated with amino-labeled DNA show a distinct Cy3 fluorescence signal, whereas DNA that was not labeled with an amino group had not bound to the surface.

Cell-Free Expression of GFP From DNA Spots

Figure 3: Fluorescent GFP spots after 30 min of cell-free expression. The fluorescence was measured by placing the assembled chamber under a microscope. The system still was filled with expression mix.

Having verified that DNA can be bound to the PDMS flow cell, the next step was showing that the immobilized sequence is still capable of being transcribed and translated.
The microfluidic chamber consisting of the PDMS slide and a glass slide with a specific Ni-NTA surface was then assembled and filled with cell-free expression mix. The expression was performed for 2 h at 37°C.
The microfluidic chamber was analyzed by fluorescence microscopy afterwards. As shown in figure 3, cell-free expressed GFP was observed in distinct spots exhibiting a clear fluorescence signal. Thus, besides being expressed, the protein was also correctly folded and remained functional.

All in all, we showed that:

  1. DNA can be immobilized reliably on a PDMS surface using an amino-label.
  2. our DNA sequences are capable of being expressed by the DiaMIX although being immobilized.
  3. the DiaMIX succeeds in the expression fully funtional GFP.