Team:Alberta/biobyte2

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==Components of the System==
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==Overview==
<div id="horiz-line"></div>
<div id="horiz-line"></div>
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The Assembly Method 2.0 is composed of three main componentsAn <b>anchor</b> byte attached to an iron micro bead is the beginning of a construct.  Because of the magnetic nature of these beads, they can be positioned by using a simple magnetThe <b>BioBytes</b> are added to the anchor-byte one at a time in sequenceThis is possible due to the alternating overhang structure of the <b>BioBytes</b>a. Finally, a <b>cap</b> is added allowing for circularization of the construct. The construct is now ready to transform
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BioBytes 2.0 is the heart of the GENOMIKON kitBioBytes 2.0 is a method of creating novel plasmids through the sequential addition of functional units of DNAIt is designed to be used in a high school setting but has potential to be used in professional settings as wellThe assembly method we have created has some conceptual similarities to the original BioBytes Assembly System developed from the 2009 Alberta iGEM project. However, there are some striking differences between the two systems.
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====Overhangs====
+
==Traditional Methods==
 +
<div id="horiz-line"></div>
 +
The current assembly standard is the BioBrick method.  While the registry of parts and the assembly standard has allowed for effective construction of plasmids in a laboratory setting, it has numerous limitations prohibiting its use in high schools.  For example, common laboratory protocols such as transformation, ligation, and restriction digestion require materials and equipment not available to high schools. Not only does this require expensive reagents and equipment, it also takes days to weeks to assemble a complicated construct. An experiment of such length far surpasses the average high school student’s attention span and the time a curriculum can spend on a particular subject.
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====Anchor Byte====
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[[Image:team-alberta-biobrick-tour.jpg|center|frame|Figure 1.1. Traditional BioBrick construction which takes approximately 3 days to complete the addition of one part; from the cutting of the original constructs to transformation and confirmation.]]
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The Anchor-byte begins the process of assembly.  It is composed of:
+
====Comparison====
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*a poly-A tail
+
The BioBytes Assembly System 2.0 has provided a solution to these issues.  The GENOMIKON kit is fast allowing for assembly of a novel plasmid in an afternoon rather than over the course of several days.  The kit is completely self-contained, requiring no other equipment or reagents that does not come with the kit. This eliminates the need for the expensive equipment and reagents common place in a University laboratory setting.
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*a BsaI recognition site
+
The addition of one part to a construct takes under 10 minutes. So creating a plasmid of your desired specifications can happen in an afternoon, rather than the 3 or more days to create a plasmid through the traditional BioBrick methods.
-
*an A or B overhang
+
 +
==Components of the System==
 +
<div id="horiz-line"></div>
-
Iron micro beads purchased from New England Biolabs have covalently attached poly-T tails. The bead allows us to manipulate the DNA with magnets making washing and subsequent attachments easier.
+
The Assembly Method 2.0 is composed of three main components.  An <b>anchor</b> piece attached to a ferro-magnetic bead is used to begin chain initiation. Because of the magnetic nature of these beads, they can be dragged to different points in the tube using a simple magnet.  The <b>BioBytes</b> are added to the anchor piece and have alternating end structures allowing them to be added in a sequential order.  Finally, a <b>cap</b> is added allowing for circularization of the construct.
-
We have designed an anchor byte which begins the process of assembly. The anchor-byte is comprised of an Anchor piece ligated to the first byte of the assembly.  Construction begins by ligating a selectable marker to the anchor. This first step allows for complete constructs to be selected for. As well, the incorporation of a BsaI cut site into the Anchor, before the first byte, gives versatility to the construct because the first byte and the rest of the construct can be removed from the anchor, and used as a Byte in and of itself. 
+
====Overhangs====
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Once the selectable marker is ligated to the first byte, we anneal the anchor-byte to the poly-T tails on the iron micro bead. We have created anchors with both varieties of ends so that assemblies can begin with any type of byte.
+
 
 +
====Anchor====
 +
 
 +
The Anchor piece begins the process of assembly.  It is composed of:
 +
 
 +
*a poly-A tail
 +
*an AB or BA cut site
 +
*a poly-T linked ferro-magnetic bead
 +
 
 +
A ferro-magnetic bead attached to a piece of DNA. This piece serves as the initial piece from which we assemble a DNA construct.  The bead allows us to manipulate the DNA with magnets making washing and subsequent attachments easier.
 +
Magnetic beads purchased from New England Biolabs have covalently attached poly-T tails.
 +
We have designed an anchor byte which begins the process of assembly. The anchor byte is comprised of a poly-A tail and one of the two overhangs discussed earlier. Construction begins by ligating a selectable marker to the anchor. This first step allows incomplete constructs to be easily selected against. Incorporation of a BsaI cut site give versatility to the construct, an advantage discussed shortly.
 +
Once the selectable marker is ligated to the first byte,we anneal the anchor to the poly-T tails on the magnetic bead. We have created anchors with both varieties of ends so that assemblies can begin with either type of byte.
The results of one of our experiments is shown here. Note that the interaction between the anchor and the bead is non-covalent. The anchor along with the construct can be separated from the bead with heat. The lefthand gel shows the process of anchoring a construct. A anchor-byte construct of 1kb is allowed to anneal to the magnetic beads. This is done in excess, and the supernatant is shown in the first lane. A subsequent wash step showed the absence of DNA, indicating that DNA construct is stably bound. The construct can be melted from the scaffold at 70 degrees Celsius. The melted construct can be seen in the last lane.
The results of one of our experiments is shown here. Note that the interaction between the anchor and the bead is non-covalent. The anchor along with the construct can be separated from the bead with heat. The lefthand gel shows the process of anchoring a construct. A anchor-byte construct of 1kb is allowed to anneal to the magnetic beads. This is done in excess, and the supernatant is shown in the first lane. A subsequent wash step showed the absence of DNA, indicating that DNA construct is stably bound. The construct can be melted from the scaffold at 70 degrees Celsius. The melted construct can be seen in the last lane.
This schematic shows the alternating addition of bytes starting from the anchor. Parts are added and ligated in an sequential fashion. Cycle time for each step was about 7 minutes. This is much faster than the Biobrick method. In on of our assemblies, we were able to create an octamer, with a total size of 12 kb. As you can see, there are some minor incomplete products.  
This schematic shows the alternating addition of bytes starting from the anchor. Parts are added and ligated in an sequential fashion. Cycle time for each step was about 7 minutes. This is much faster than the Biobrick method. In on of our assemblies, we were able to create an octamer, with a total size of 12 kb. As you can see, there are some minor incomplete products.  
-
If you recall, we have incorporated a BsaI cut site into the anchor. This allows for constructs to be created in parallel and then utilized as large Bytes in the assembly in the same way.  
+
If you recall, we have incorporated a BsaI cut site into the anchor. This allows for constructs to be created in parallel and then utilized in the standard assembly.  
====BioBytes====
====BioBytes====
====Cap====
====Cap====
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==Byte Construction==
 +
<div id="horiz-line"></div>
 +
==Assembly System==
 +
<div id="horiz-line"></div>
 +
 +
==BioBytes Vs BioBytes 2.0==
 +
<div id="horiz-line"></div>
 +
 +
 +
The "BioBytes Version 2.0" construction method has been shown to create (insert actual data here) plasmids from up to 8 separate parts in
 +
an afternoon's work. This is a vast improvement.
 +
 +
[[Image:team-alberta-building-tour.jpg|center|frame|BioByte version 2.0 construction.]
 +
 +
==BioBytes Components==
 +
<div id="horiz-line"></div>
 +
 +
The method has three main components:
 +
 +
====The Anchor====
 +
 +
[[Image:team-alberta-anchor-tour.jpg|center|frame|The two components of the anchoring system.]]
 +
====The BioBytes====
 +
DNA fragments that can be attached together to build up a larger construct. There are two types  of pieces, AB and BA.  The A end can join only with another A end and the B end can join only with another B end.  As a result pieces can only be joined in a single orientation.
 +
[[Image:team-alberta-bytes-tour.jpg|500px|center|thumb|BioBytes come in two flavors: 'AB' and 'BA'.]]
 +
 +
 +
====The Cap====
 +
A DNA fragment that finishes off a construct and allows for circularization of the construct into a plasmid.
 +
 +
The process of building a plasmid is more elegant and more rapid than the current biobyte system! 
 +
[[Image:team-alberta-cap-tour.jpg|center|The cap. The poly-T anneals to the poly-A of the anchor component to circularize the complete plasmid.]]
 +
 +
==The Process==
 +
<div id="horiz-line"></div>
 +
[[Image:team-alberta-biobyteprocess-tour.jpg|center|frame|The entire construction process can be completed in an afternoon.]]
 +
Starting with an anchor, add the first piece and ligate.
 +
 +
Then hold the single piece construct in the tube by placing it on the magnetic rack.  Now you can wash away most of the excess of piece 1.
 +
 +
Add the next piece and repeat until you have added all the pieces you want.
 +
 +
Then add the cap.
 +
 +
Now just heat to release the anchor and open up the cap, upon cooling the construct will circularize. 
 +
 +
Easy!
 +
 +
Using this process we were able to assemble eight pieces in an afternoon!
 +
{{Team:Alberta/endMainContent|class=not-top}}

Revision as of 00:45, 27 October 2010

TEAM ALBERTA

Overview

BioBytes 2.0 is the heart of the GENOMIKON kit. BioBytes 2.0 is a method of creating novel plasmids through the sequential addition of functional units of DNA. It is designed to be used in a high school setting but has potential to be used in professional settings as well. The assembly method we have created has some conceptual similarities to the original BioBytes Assembly System developed from the 2009 Alberta iGEM project. However, there are some striking differences between the two systems.

Traditional Methods

The current assembly standard is the BioBrick method. While the registry of parts and the assembly standard has allowed for effective construction of plasmids in a laboratory setting, it has numerous limitations prohibiting its use in high schools. For example, common laboratory protocols such as transformation, ligation, and restriction digestion require materials and equipment not available to high schools. Not only does this require expensive reagents and equipment, it also takes days to weeks to assemble a complicated construct. An experiment of such length far surpasses the average high school student’s attention span and the time a curriculum can spend on a particular subject.


Figure 1.1. Traditional BioBrick construction which takes approximately 3 days to complete the addition of one part; from the cutting of the original constructs to transformation and confirmation.

Comparison

The BioBytes Assembly System 2.0 has provided a solution to these issues. The GENOMIKON kit is fast allowing for assembly of a novel plasmid in an afternoon rather than over the course of several days. The kit is completely self-contained, requiring no other equipment or reagents that does not come with the kit. This eliminates the need for the expensive equipment and reagents common place in a University laboratory setting. The addition of one part to a construct takes under 10 minutes. So creating a plasmid of your desired specifications can happen in an afternoon, rather than the 3 or more days to create a plasmid through the traditional BioBrick methods.

Components of the System

The Assembly Method 2.0 is composed of three main components. An anchor piece attached to a ferro-magnetic bead is used to begin chain initiation. Because of the magnetic nature of these beads, they can be dragged to different points in the tube using a simple magnet. The BioBytes are added to the anchor piece and have alternating end structures allowing them to be added in a sequential order. Finally, a cap is added allowing for circularization of the construct.

Overhangs

Anchor

The Anchor piece begins the process of assembly. It is composed of:

  • a poly-A tail
  • an AB or BA cut site
  • a poly-T linked ferro-magnetic bead

A ferro-magnetic bead attached to a piece of DNA. This piece serves as the initial piece from which we assemble a DNA construct. The bead allows us to manipulate the DNA with magnets making washing and subsequent attachments easier. Magnetic beads purchased from New England Biolabs have covalently attached poly-T tails. We have designed an anchor byte which begins the process of assembly. The anchor byte is comprised of a poly-A tail and one of the two overhangs discussed earlier. Construction begins by ligating a selectable marker to the anchor. This first step allows incomplete constructs to be easily selected against. Incorporation of a BsaI cut site give versatility to the construct, an advantage discussed shortly. Once the selectable marker is ligated to the first byte,we anneal the anchor to the poly-T tails on the magnetic bead. We have created anchors with both varieties of ends so that assemblies can begin with either type of byte. The results of one of our experiments is shown here. Note that the interaction between the anchor and the bead is non-covalent. The anchor along with the construct can be separated from the bead with heat. The lefthand gel shows the process of anchoring a construct. A anchor-byte construct of 1kb is allowed to anneal to the magnetic beads. This is done in excess, and the supernatant is shown in the first lane. A subsequent wash step showed the absence of DNA, indicating that DNA construct is stably bound. The construct can be melted from the scaffold at 70 degrees Celsius. The melted construct can be seen in the last lane.

This schematic shows the alternating addition of bytes starting from the anchor. Parts are added and ligated in an sequential fashion. Cycle time for each step was about 7 minutes. This is much faster than the Biobrick method. In on of our assemblies, we were able to create an octamer, with a total size of 12 kb. As you can see, there are some minor incomplete products.

If you recall, we have incorporated a BsaI cut site into the anchor. This allows for constructs to be created in parallel and then utilized in the standard assembly.

BioBytes

Cap

Byte Construction

Assembly System

BioBytes Vs BioBytes 2.0


The "BioBytes Version 2.0" construction method has been shown to create (insert actual data here) plasmids from up to 8 separate parts in an afternoon's work. This is a vast improvement.

[[Image:team-alberta-building-tour.jpg|center|frame|BioByte version 2.0 construction.]

BioBytes Components

The method has three main components:

The Anchor

The two components of the anchoring system.

The BioBytes

DNA fragments that can be attached together to build up a larger construct. There are two types of pieces, AB and BA. The A end can join only with another A end and the B end can join only with another B end. As a result pieces can only be joined in a single orientation.

BioBytes come in two flavors: 'AB' and 'BA'.


The Cap

A DNA fragment that finishes off a construct and allows for circularization of the construct into a plasmid.

The process of building a plasmid is more elegant and more rapid than the current biobyte system!

The cap. The poly-T anneals to the poly-A of the anchor component to circularize the complete plasmid.

The Process

The entire construction process can be completed in an afternoon.

Starting with an anchor, add the first piece and ligate.

Then hold the single piece construct in the tube by placing it on the magnetic rack. Now you can wash away most of the excess of piece 1.

Add the next piece and repeat until you have added all the pieces you want.

Then add the cap.

Now just heat to release the anchor and open up the cap, upon cooling the construct will circularize.

Easy!

Using this process we were able to assemble eight pieces in an afternoon!