Team:Johns Hopkins/Notebook/GROUP 2: MATa Specific-promoters

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(Difference between revisions)
(GROUP 2: MATa Specific-promoters)
(GROUP 2: MATa Specific-promoters)
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== GROUP 2: MATa Specific-promoters ==
== GROUP 2: MATa Specific-promoters ==
-
   Status report by Allison and Nate
+
  Date: August 12, 2008
-
   Part no.: BBa_K110008
+
   Status report by: Allison and Nate
-
   Part Description: MFA1 (L+R)
+
   Part no.: BBa_K11008 -> BBa_K110016
-
   Part Location: in a labeled box, second shelf from the top, -20
+
   Part Description: A promoters MFA1 (L+R) and Ste2 (R+L)
-
  degrees C refrigerator next to front door
+
   '''Two more minipreps were completed. DNA concentrations were much higher (>150 ng/ul).'''
-
   Date: 7/10/08
+
 
-
   PCR successful? Yes
+
   Date: August 5, 2008
-
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16]
+
   Status report by: Allison and Nate
-
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016%20Using%20Constant%20Annealing.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16 Using Constant Annealing]
+
   Part no.: BBa_K110008 -> BBa_K110016
-
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Short%202Way%20Stop,%20Alpha%20Promoters,%20&%20Sapphire%20FP.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Short 2Way Stop, Alpha Promoters, & Sapphire FP]
+
   Part Description: A promoters: MFA1 (L+R) and Ste2 (R+L), respectively.
-
   Cloning of PCR product successful: in progress
+
   <b>Sequences were analyzed. BBa_K110016 had a perfect clone. Since there is not much
-
   Sequencing of cloned PCR product successful: not done
+
  miniprep left, a transformation will be done to generate more clones with the
-
   Joining of validated part to adjacent part(s) status: not done
+
  correct sequence. BBa_K110008 had one mutation; additional minipreps from other clones
-
   Problems to be solved: to be determined
+
  are ready to send off for sequencing, although the DNA concentrations are low. Colonies
-
   Current status of this part: PCR was being troubleshooted, appeared to
+
   can be picked and overnight cultures grown
-
   have good results with regular PCR protocol (not touchdown) in which
+
   for another round of minipreps.</b>
-
   there was a constant annealing temperature of 55 degrees C - see gel
+
 
 +
   Date: July 29, 2008
 +
   Status report by: Allison and Nate
 +
   Part no.: BBa_K110008 -> BBa_K110016
 +
   Part Description: A promoters: MFA1 (L+R) and Ste2 (R+L), respectively.
 +
   <b>Two samples of mini preps from MFA1 and Ste2 were sent off for sequencing at the end of last week.
 +
  Results will follow soon.</b>
   Status report by Allison and Nate
   Status report by Allison and Nate
   Part no.: BBa_K110016
   Part no.: BBa_K110016
   Part Description: Ste2 (R+L)
   Part Description: Ste2 (R+L)
-
   Part Location: in a labeled box, second shelf from the top, -20
+
   Part Location: in a labeled box, second shelf from the top, -20 degrees C refrigerator next to  
-
  degrees C refrigerator next to front door
+
  front door; plates at 4 degrees
-
   Date: 7/10/08
+
   Date: 7/22/08
   PCR successful? Yes
   PCR successful? Yes
-
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16]
+
   <b>Cloning of PCR product successful: Yes (approx 20 white colonies on one plate)</b>
-
  [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016%20Using%20Constant%20Annealing.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16 Using Constant Annealing]
+
-
  [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Short%202Way%20Stop,%20Alpha%20Promoters,%20&%20Sapphire%20FP.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Short 2Way Stop, Alpha Promoters, & Sapphire FP]
+
-
  Cloning of PCR product successful: in progress
+
-
  Sequencing of cloned PCR product successful: not done
+
   Joining of validated part to adjacent part(s) status: not done
   Joining of validated part to adjacent part(s) status: not done
-
   Problems to be solved: to be determined
+
   Problems to be solved:
-
   Current status of this part: Both PCR protocols (touchdown and second
+
   <b>Current status of this part: 12 mini preps and the restriction digestion were completed;
-
  PCR with constant annealing temperature) produced product of the
+
   preparing to send 3 samples to be sequenced
-
   correct size. BBa_K110016 was used as a control in the second PCR with
+
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Restriction%20Digests%20of%20BBa_K1100...%2008%20&%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Restriction Digests of BBa_K1100... 08 & 16]</b>
-
   BBa_K110008.
+
   Status report by Allison and Nate
   Status report by Allison and Nate
Line 44: Line 45:
   Part Description: MFA1 (L+R)
   Part Description: MFA1 (L+R)
   Part Location: same as above, plates are at 4 degrees refrigerator near front door
   Part Location: same as above, plates are at 4 degrees refrigerator near front door
-
   Date: 7/14/08
+
   Date: 7/22/08
-
   PCR successful? Yes
+
   <b>PCR successful? Yes  
-
   Cloning of PCR product of successful? There were mainly light blue colonies
+
  (BAD LINK)
-
  (only a couple white colonies)
+
   Cloning of PCR product of successful? Yes (approx 60 white colonies between two plates)</b>
   Sequencing of cloned PCR product successful: not done
   Sequencing of cloned PCR product successful: not done
   Joining of validated part to adjacent part(s) status: not done
   Joining of validated part to adjacent part(s) status: not done
-
   Problems to be solved: Ligation
+
   Problems to be solved:
-
   Current status of this part: plates are at 4 degrees; another ligation/transformation
+
   <b>Current status of this part: 12 mini preps and the restriction digestion were completed;</b>
-
  will be completed soon
+
  <b>preparing to send 3 samples to be sequenced
 +
  [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Restriction%20Digests%20of%20BBa_K1100...%2008%20&%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Restriction Digests of BBa_K1100... 08 & 16]</b>
   Status report by Allison and Nate
   Status report by Allison and Nate
Line 72: Line 74:
   Part Description: MFA1 (L+R)
   Part Description: MFA1 (L+R)
   Part Location: same as above, plates are at 4 degrees refrigerator near front door
   Part Location: same as above, plates are at 4 degrees refrigerator near front door
-
   Date: 7/22/08
+
   Date: 7/14/08
-
   <b>PCR successful? Yes  
+
   PCR successful? Yes
-
  (BAD LINK)
+
   Cloning of PCR product of successful? There were mainly light blue colonies
-
   Cloning of PCR product of successful? Yes (approx 60 white colonies between two plates)</b>
+
  (only a couple white colonies)
   Sequencing of cloned PCR product successful: not done
   Sequencing of cloned PCR product successful: not done
   Joining of validated part to adjacent part(s) status: not done
   Joining of validated part to adjacent part(s) status: not done
-
   Problems to be solved:
+
   Problems to be solved: Ligation
-
   <b>Current status of this part: 12 mini preps and the restriction digestion were completed;</b>
+
   Current status of this part: plates are at 4 degrees; another ligation/transformation
-
  <b>preparing to send 3 samples to be sequenced
+
  will be completed soon
-
  [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Restriction%20Digests%20of%20BBa_K1100...%2008%20&%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Restriction Digests of BBa_K1100... 08 & 16]</b>
+
   Status report by Allison and Nate
   Status report by Allison and Nate
   Part no.: BBa_K110016
   Part no.: BBa_K110016
   Part Description: Ste2 (R+L)
   Part Description: Ste2 (R+L)
-
   Part Location: in a labeled box, second shelf from the top, -20 degrees C refrigerator next to  
+
   Part Location: in a labeled box, second shelf from the top, -20
-
  front door; plates at 4 degrees
+
  degrees C refrigerator next to front door
-
   Date: 7/22/08
+
   Date: 7/10/08
   PCR successful? Yes
   PCR successful? Yes
-
   <b>Cloning of PCR product successful: Yes (approx 20 white colonies on one plate)</b>
+
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16]
 +
  [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016%20Using%20Constant%20Annealing.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16 Using Constant Annealing]
 +
  [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Short%202Way%20Stop,%20Alpha%20Promoters,%20&%20Sapphire%20FP.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Short 2Way Stop, Alpha Promoters, & Sapphire FP]
 +
  Cloning of PCR product successful: in progress
 +
  Sequencing of cloned PCR product successful: not done
   Joining of validated part to adjacent part(s) status: not done
   Joining of validated part to adjacent part(s) status: not done
-
   Problems to be solved:
+
   Problems to be solved: to be determined
-
   <b>Current status of this part: 12 mini preps and the restriction digestion were completed;
+
   Current status of this part: Both PCR protocols (touchdown and second
-
   preparing to send 3 samples to be sequenced
+
  PCR with constant annealing temperature) produced product of the
-
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Restriction%20Digests%20of%20BBa_K1100...%2008%20&%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Restriction Digests of BBa_K1100... 08 & 16]</b>
+
   correct size. BBa_K110016 was used as a control in the second PCR with
 +
   BBa_K110008.
-
  Date: July 29, 2008
+
   Status report by Allison and Nate
-
   Status report by: Allison and Nate
+
   Part no.: BBa_K110008
-
   Part no.: BBa_K110008 -> BBa_K110016
+
   Part Description: MFA1 (L+R)
-
   Part Description: A promoters: MFA1 (L+R) and Ste2 (R+L), respectively.
+
   Part Location: in a labeled box, second shelf from the top, -20
-
   <b>Two samples of mini preps from MFA1 and Ste2 were sent off for sequencing at the end of last week.
+
   degrees C refrigerator next to front door
-
   Results will follow soon.</b>
+
   Date: 7/10/08
-
 
+
   PCR successful? Yes
-
   Date: August 5, 2008
+
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16]
-
   Status report by: Allison and Nate
+
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016%20Using%20Constant%20Annealing.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16 Using Constant Annealing]
-
   Part no.: BBa_K110008 -> BBa_K110016
+
   [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Short%202Way%20Stop,%20Alpha%20Promoters,%20&%20Sapphire%20FP.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Short 2Way Stop, Alpha Promoters, & Sapphire FP]
-
   Part Description: A promoters: MFA1 (L+R) and Ste2 (R+L), respectively.
+
   Cloning of PCR product successful: in progress
-
   <b>Sequences were analyzed. BBa_K110016 had a perfect clone. Since there is not much
+
   Sequencing of cloned PCR product successful: not done
-
  miniprep left, a transformation will be done to generate more clones with the
+
   Joining of validated part to adjacent part(s) status: not done
-
  correct sequence. BBa_K110008 had one mutation; additional minipreps from other clones
+
   Problems to be solved: to be determined
-
  are ready to send off for sequencing, although the DNA concentrations are low. Colonies
+
   Current status of this part: PCR was being troubleshooted, appeared to
-
   can be picked and overnight cultures grown
+
   have good results with regular PCR protocol (not touchdown) in which
-
   for another round of minipreps.</b>
+
   there was a constant annealing temperature of 55 degrees C - see gel
-
 
+
-
   Date: August 12, 2008
+
-
   Status report by: Allison and Nate
+
-
   Part no.: BBa_K11008 -> BBa_K110016
+
-
   Part Description: A promoters MFA1 (L+R) and Ste2 (R+L)
+
-
   '''Two more minipreps were completed. DNA concentrations were much higher (>150 ng/ul).'''
+

Revision as of 01:30, 13 August 2008

GROUP 2: MATa Specific-promoters

 Date: August 12, 2008
 Status report by: Allison and Nate
 Part no.: BBa_K11008 -> BBa_K110016
 Part Description: A promoters MFA1 (L+R) and Ste2 (R+L)
 Two more minipreps were completed. DNA concentrations were much higher (>150 ng/ul).
 Date: August 5, 2008
 Status report by: Allison and Nate
 Part no.: BBa_K110008 -> BBa_K110016
 Part Description: A promoters: MFA1 (L+R) and Ste2 (R+L), respectively.
 Sequences were analyzed. BBa_K110016 had a perfect clone. Since there is not much
 miniprep left, a transformation will be done to generate more clones with the 
 correct sequence. BBa_K110008 had one mutation; additional minipreps from other clones
 are ready to send off for sequencing, although the DNA concentrations are low. Colonies
 can be picked and overnight cultures grown
 for another round of minipreps.
 Date: July 29, 2008
 Status report by: Allison and Nate
 Part no.: BBa_K110008 -> BBa_K110016
 Part Description: A promoters: MFA1 (L+R) and Ste2 (R+L), respectively.
 Two samples of mini preps from MFA1 and Ste2 were sent off for sequencing at the end of last week.
 Results will follow soon.
 Status report by Allison and Nate
 Part no.: BBa_K110016
 Part Description: Ste2 (R+L)
 Part Location: in a labeled box, second shelf from the top, -20 degrees C refrigerator next to 
  front door; plates at 4 degrees
 Date: 7/22/08
 PCR successful? Yes
 Cloning of PCR product successful: Yes (approx 20 white colonies on one plate)
 Joining of validated part to adjacent part(s) status: not done
 Problems to be solved:
 Current status of this part: 12 mini preps and the restriction digestion were completed;
 preparing to send 3 samples to be sequenced
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Restriction%20Digests%20of%20BBa_K1100...%2008%20&%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Restriction Digests of BBa_K1100... 08 & 16]
 Status report by Allison and Nate
 Part no.: BBa_K110008
 Part Description: MFA1 (L+R)
 Part Location: same as above, plates are at 4 degrees refrigerator near front door
 Date: 7/22/08
 PCR successful? Yes 
 (BAD LINK)
 Cloning of PCR product of successful? Yes (approx 60 white colonies between two plates)
 Sequencing of cloned PCR product successful: not done
 Joining of validated part to adjacent part(s) status: not done
 Problems to be solved:
 Current status of this part: 12 mini preps and the restriction digestion were completed;
 preparing to send 3 samples to be sequenced
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Restriction%20Digests%20of%20BBa_K1100...%2008%20&%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Restriction Digests of BBa_K1100... 08 & 16]
 Status report by Allison and Nate
 Part no.: BBa_K110016
 Part Description: Ste2 (R+L)
 Part Location: in a labeled box, second shelf from the top, -20 degrees C refrigerator next to 
  front door; plates at 4 degrees
 Date: 7/14/08
 PCR successful? Yes
 Cloning of PCR product successful: There were many blue colonies (similar to the plate of BB_K110008)
 Sequencing of cloned PCR product successful: not done
 Joining of validated part to adjacent part(s) status: not done
 Problems to be solved: Ligation
 Current status of this part: plates are at 4 degrees; another ligation/transformation 
  will be completed soon
 Status report by Allison and Nate
 Part no.: BBa_K110008
 Part Description: MFA1 (L+R)
 Part Location: same as above, plates are at 4 degrees refrigerator near front door
 Date: 7/14/08
 PCR successful? Yes
 Cloning of PCR product of successful? There were mainly light blue colonies 
  (only a couple white colonies)
 Sequencing of cloned PCR product successful: not done
 Joining of validated part to adjacent part(s) status: not done
 Problems to be solved: Ligation
 Current status of this part: plates are at 4 degrees; another ligation/transformation 
  will be completed soon
 Status report by Allison and Nate
 Part no.: BBa_K110016
 Part Description: Ste2 (R+L)
 Part Location: in a labeled box, second shelf from the top, -20
 degrees C refrigerator next to front door
 Date: 7/10/08
 PCR successful? Yes
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16]
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016%20Using%20Constant%20Annealing.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16 Using Constant Annealing]
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Short%202Way%20Stop,%20Alpha%20Promoters,%20&%20Sapphire%20FP.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Short 2Way Stop, Alpha Promoters, & Sapphire FP]
 Cloning of PCR product successful: in progress
 Sequencing of cloned PCR product successful: not done
 Joining of validated part to adjacent part(s) status: not done
 Problems to be solved: to be determined
 Current status of this part: Both PCR protocols (touchdown and second
 PCR with constant annealing temperature) produced product of the
 correct size. BBa_K110016 was used as a control in the second PCR with
 BBa_K110008.
 Status report by Allison and Nate
 Part no.: BBa_K110008
 Part Description: MFA1 (L+R)
 Part Location: in a labeled box, second shelf from the top, -20
 degrees C refrigerator next to front door
 Date: 7/10/08
 PCR successful? Yes
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16]
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.BioBricks%208%20and%2016%20Using%20Constant%20Annealing.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html BioBricks 8 and 16 Using Constant Annealing]
 [http://www.jhu.edu/iGEM/Group2:MATaSpecificPromoters/2008-7-22.Short%202Way%20Stop,%20Alpha%20Promoters,%20&%20Sapphire%20FP.Allison%20Suarez%20and%20Nate%20Sotuyo%20.html Short 2Way Stop, Alpha Promoters, & Sapphire FP]
 Cloning of PCR product successful: in progress
 Sequencing of cloned PCR product successful: not done
 Joining of validated part to adjacent part(s) status: not done
 Problems to be solved: to be determined
 Current status of this part: PCR was being troubleshooted, appeared to
 have good results with regular PCR protocol (not touchdown) in which
 there was a constant annealing temperature of 55 degrees C - see gel