Difference between revisions of "Part:BBa K349005"

(Usage and Biology)
 
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<partinfo>BBa_K349005 short</partinfo>
 
<partinfo>BBa_K349005 short</partinfo>
  
Base plasmid v.2 for the construction of parts compatible with the BioBytes 2.0 assembly method.  The RFP cassette can be removed using the BfuAI enzyme and a new AB ORF style may be inserted into the plasmid allowing for creation of the parts for the BioBytes 2.0 assembly method.
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This is the RFP BfuAI AB Base Plasmid v.2 for the construction of components of Team Alberta's 2010 BioBytes 2.0 assembly method. The RFP cassette can be removed using the BfuAI enzyme and a new part may be inserted into the plasmid in order to amplify it in the AB Byte format applicable to this method.
 
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__NOTOC__
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<partinfo>BBa_K349001 short</partinfo>
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This is the RFP BsaI AB Base Plasmid v.2 for the construction of components of Team Alberta's 2010 BioBytes 2.0 assembly method. The RFP cassette can be removed using the BsaI enzyme and a new part may be inserted into the plasmid in order to amplify it in the AB Byte format applicable to this method.
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This plasmid is a useful tool for creating AB Bytes in compliance with the BioBytes 2.0 assembly method according to the following procedure:
 
This plasmid is a useful tool for creating AB Bytes in compliance with the BioBytes 2.0 assembly method according to the following procedure:
  
1) PCR the part of interest, incorporating BsaI cut sites with appropriate overhangs onto each side. For more information on these overhangs click <html><a href="http://2010.igem.org/Team:Alberta/biobyte2">here.</a></html>  
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1) PCR the part of interest, incorporating BfuAI cut sites with appropriate overhangs onto each side. For more information on these overhangs click <html><a href="http://2010.igem.org/Team:Alberta/biobyte2">here.</a></html>  
  
2) Digest both this RFP BsaI AB Base Plasmid (v.2) and the PCR product with BsaI.  
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2) Digest both this RFP BfuAI AB Base Plasmid (v.2) and the PCR product with BfuAI.  
  
 
3) Ligate them together. Because the overhangs are unique, the plasmid backbone can not re-ligate without an insert. The insert can only be the new part of interest, or the RFP coding cassette that was originally in the base plasmid, leading to a total of 2 possible ligation products.  
 
3) Ligate them together. Because the overhangs are unique, the plasmid backbone can not re-ligate without an insert. The insert can only be the new part of interest, or the RFP coding cassette that was originally in the base plasmid, leading to a total of 2 possible ligation products.  
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Biobytes 2.0 Assembly Protocol:
 
Biobytes 2.0 Assembly Protocol:
  
When digested with BsaI and purified, this plasmid can yield an AB RFP cassette. It can also be used to make other AB Bytes as per the process described above and subsequently digested with BsaI and purified to yield those particular AB Bytes. Certain Bytes can be added together sequentially using the BioBytes 2.0 assembly method. For a detailed overview of this method, click <html><a href="http://2010.igem.org/Team:Alberta/biobyte2">here.</a></html> The following protocol summarizes the steps involved in multiple Byte assembly: <br>
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When digested with BfuAI and purified, this plasmid can yield an AB RFP cassette. It can also be used to make other AB Bytes as per the process described above and subsequently digested with BsaI and purified to yield those particular AB Bytes. Certain Bytes can be added together sequentially using the BioBytes 2.0 assembly method. For a detailed overview of this method, click <html><a href="http://2010.igem.org/Team:Alberta/biobyte2">here.</a></html> The following protocol summarizes the steps involved in multiple Byte assembly: <br>
  
 
1) Mix the iron micro beads for 10 minutes.<br>
 
1) Mix the iron micro beads for 10 minutes.<br>
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19) After the last Byte has been ligated and washed, add 30 ul of 75C Elution Buffer. Keep at 75C for 10 minutes. <br>
 
19) After the last Byte has been ligated and washed, add 30 ul of 75C Elution Buffer. Keep at 75C for 10 minutes. <br>
 
20) After 10  minutes, still at 75C, put the tube into a magnetic rack . Allow the beads to be pulled aside and collect the supernatant into a clean 1.5 mL tube. The supernatant will contain your construct. <br>
 
20) After 10  minutes, still at 75C, put the tube into a magnetic rack . Allow the beads to be pulled aside and collect the supernatant into a clean 1.5 mL tube. The supernatant will contain your construct. <br>
 
  
 
===Characterization===
 
===Characterization===
The successful characterization of this part entails demonstrating its utility in the creation of new AB Bytes, because this plasmid was designed to be a base plasmid for the production of all AB bytes. The following point summarize the effectiveness of this part.
 
 
(I) RFP AB BsaI plasmid was successfully transformed, resulting in red fluorescent colonies on LB medium.
 
[[Image:Alberta2010LBORFP.jpg|200px|center|frame|RFP AB-BsaI plasmids growing on LBO (LB medium).]]
 
 
(II)The RFP cassette of this plasmid was sequence-verified. It contained the proper A and B overhangs, BsaI recognition sites, BioBrick prefix and suffix and proper ORF sequences.
 
  
(III)The plasmid was cut with BsaI and showed a gel similar to that seen for the [https://parts.igem.org/wiki/index.php?title=Part:BBa_K349007 KanR plasmids]
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(I) RFP AB BfuAI plasmid was successfully transformed, resulting in red fluorescent colonies similar to those of <html><a href="https://parts.igem.org/Part:BBa_K349001">BBa_K349001</a></html>.
  
(IV)BsaI cutting efficiency and fidelity was confirmed in its use in creating other AB parts. This plasmid was used to create most AB Bytes by Team Alberta following the protocol for creating new AB bytes described above. The procedure was performed using crtE, and resulted in red and white colonies on the plate, as expected. For an indepth view of these experiments, click <html><a href="http://2010.igem.org/wiki/index.php?title=Team:Alberta/Notebook/BasePlasmids">here.</a></html>
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(II)The plasmid was cut with BfuAI and produced expected size fragments similar to those of <html><a href="https://parts.igem.org/Part:BBa_K349001">BBa_K349002</a></html>.
[[Image:Alberta2010makingparts3.jpg|200px|center|frame|White and red colonies produced when making parts using RFP BsaI AB Base Plasmid v.2.]]
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(V) kan AB Bytes and the original RFP AB Byte from this plasmid were used to test the effectiveness of the assembly of multiple bytes. An anchor-KanR(AB)-Ori-RFP(AB)-Cap construct was made using the procedure described above and then it was allowed to recircularize. Numerous red fluorescent colonies were present on kanamycin LB plates the following day.  
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(III)BfuAI cutting efficiency and fidelity was confirmed in its use in creating other AB parts. This plasmid was used to create mWasabi, and resulted in white and red colonies on the plate, as expected. Minipreps were made from the white colonies that yielded correct size bands after BsaI digestion. For an indepth view of this experiment, visit the section <html><a href="http://2010.igem.org/wiki/index.php?title=Team:Alberta/Notebook/BasePlasmids">Selecting Colonies with our Plasmid.</a></html>
[[Image:Alberta Rfpkan.jpg|200px|center|frame|Red fluorescent colonies produced from a 5 piece Byte construction using the BioBytes 2.0 assembly method.]]
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Together, this data demonstrates that the RFP cassette itself is functional, that the plasmid can be used to create other AB bytes, and that AB bytes made from through this plasmid function properly in our multiple-Byte assembly method.  
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Together, this data demonstrates that the RFP cassette itself is functional, cuts correctly and that the plasmid can be used to create other AB bytes.  
  
  
  
 
<span class='h3bb'>Sequence and Features</span>
 
<span class='h3bb'>Sequence and Features</span>
<partinfo>BBa_K349001 SequenceAndFeatures</partinfo>
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<partinfo>BBa_K349005 SequenceAndFeatures</partinfo>
  
  
 
<!-- Uncomment this to enable Functional Parameter display  
 
<!-- Uncomment this to enable Functional Parameter display  
 
===Functional Parameters===
 
===Functional Parameters===
<partinfo>BBa_K349001 parameters</partinfo>
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<partinfo>BBa_K349005 parameters</partinfo>
 
<!-- -->
 
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Latest revision as of 19:36, 11 August 2011

RFP-AB-BfuAI (for construction of AB BioBytes 2.0)

This is the RFP BfuAI AB Base Plasmid v.2 for the construction of components of Team Alberta's 2010 BioBytes 2.0 assembly method. The RFP cassette can be removed using the BfuAI enzyme and a new part may be inserted into the plasmid in order to amplify it in the AB Byte format applicable to this method.


Usage and Biology

This plasmid is a useful tool for creating AB Bytes in compliance with the BioBytes 2.0 assembly method according to the following procedure:

1) PCR the part of interest, incorporating BfuAI cut sites with appropriate overhangs onto each side. For more information on these overhangs click here.

2) Digest both this RFP BfuAI AB Base Plasmid (v.2) and the PCR product with BfuAI.

3) Ligate them together. Because the overhangs are unique, the plasmid backbone can not re-ligate without an insert. The insert can only be the new part of interest, or the RFP coding cassette that was originally in the base plasmid, leading to a total of 2 possible ligation products.

4) When transformed, the ligation products can appear red (if the original RFP cassette is reinserted) or white (if the part of interest is inserted). This provides a selection method for plasmids that have the part of interest in it.


Biobytes 2.0 Assembly Protocol:

When digested with BfuAI and purified, this plasmid can yield an AB RFP cassette. It can also be used to make other AB Bytes as per the process described above and subsequently digested with BsaI and purified to yield those particular AB Bytes. Certain Bytes can be added together sequentially using the BioBytes 2.0 assembly method. For a detailed overview of this method, click here. The following protocol summarizes the steps involved in multiple Byte assembly:

1) Mix the iron micro beads for 10 minutes.
2) Transfer 20 ul of iron micro beads to a 1.5 mL tube.
3) Pull the beads to the side using a magnetic tube rack.
4) Remove and discard the supernatant.
5) Add 50 ul of BioBytes 2.0 Wash Buffer to the beads. Flick gently to resuspend.
6) Pull the beads to the side using a magnetic tube rack.
7) Remove and discard the supernatant.
8) Repeat steps 5 to 7.
9) Add 200 ng of a premade anchor-Byte construct (premade in the GENOMIKON kit) to the beads and top off the volume to 20ul with TE Buffer. Flick gently to resuspend.
10) Allow annealing for 30 minutes, mixing by flicking every 5 minutes. Ensure that there are no droplets on the sides of the tube.
11) Repeat steps 6 and 7.
12) Repeat steps 5 to 7.
13) Add 200 ng of the next BioByte of your construct, making sure that a BA Byte follows an AB Byte and vice versa. Add an appropriate amount of 2x QuickLigase Buffer, Quick Ligase and TE to a total volume of 20ul.
14) Flick gently to resuspend. Allow ligation for five minutes, flicking gently every minute.
15) Add 30ul of Wash Buffer to the tube. Flick gently.
16) Repeats steps 6 and 7.
17) Repeat steps 5 to 7 twice.
18) Repeat steps 13 to 17 for each subsequent Byte addition, including the last BioByte.
19) After the last Byte has been ligated and washed, add 30 ul of 75C Elution Buffer. Keep at 75C for 10 minutes.
20) After 10 minutes, still at 75C, put the tube into a magnetic rack . Allow the beads to be pulled aside and collect the supernatant into a clean 1.5 mL tube. The supernatant will contain your construct.

Characterization

(I) RFP AB BfuAI plasmid was successfully transformed, resulting in red fluorescent colonies similar to those of BBa_K349001.

(II)The plasmid was cut with BfuAI and produced expected size fragments similar to those of BBa_K349002.

(III)BfuAI cutting efficiency and fidelity was confirmed in its use in creating other AB parts. This plasmid was used to create mWasabi, and resulted in white and red colonies on the plate, as expected. Minipreps were made from the white colonies that yielded correct size bands after BsaI digestion. For an indepth view of this experiment, visit the section Selecting Colonies with our Plasmid.


Together, this data demonstrates that the RFP cassette itself is functional, cuts correctly and that the plasmid can be used to create other AB bytes.


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]