Team:The University of Alberta/13 June 2008

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*Developed the Westerns after an overnight exposure. Blank yet again. James thought the problem was due to the development solution used - it was an old tube in the fridge that had been mixed months ago and was probably no good anymore. New solution was made and applied, film was exposed for 60 seconds and again, there were no results. This is odd because there were obvious thick bands of overexpressed proteins when we did the Coomassie staining. We will need to set up some cultures when we use the Ni-NTA columns so perhaps we will do them in duplicate and use one set for Westerns again.
*Developed the Westerns after an overnight exposure. Blank yet again. James thought the problem was due to the development solution used - it was an old tube in the fridge that had been mixed months ago and was probably no good anymore. New solution was made and applied, film was exposed for 60 seconds and again, there were no results. This is odd because there were obvious thick bands of overexpressed proteins when we did the Coomassie staining. We will need to set up some cultures when we use the Ni-NTA columns so perhaps we will do them in duplicate and use one set for Westerns again.
*Digested I725021,I725022,I725025 and I725099 with xbal and pst
*Digested I725021,I725022,I725025 and I725099 with xbal and pst
-
*Did miniprep on Tom's 2 night+ 1 day "overnight", did get a high yeild of DNA, so tried to run them on a gel.
+
*Did miniprep on Tom's 2 night+ 1 day "overnight", didn't get a high yeild of DNA, so tried to run them on a gel.
 +
*Got results back from Winnie's sequencing of the old Blue Ox biobrick. The sequences look good but they dont match the reference sequences <u>at all</u>. Dunno what's going on here but it probably doesn't matter because we are remaking all of the bricks anyway.
==Lab Tip of the Day==
==Lab Tip of the Day==
When you do a digest, make sure you label the tubes clearly and be sure to include the name of the enzymes you used to do the digest. Since the BioBricks make use of multiple enzymes, it is important to know what has been digested with which, so the parts will fit together properly upon ligation.
When you do a digest, make sure you label the tubes clearly and be sure to include the name of the enzymes you used to do the digest. Since the BioBricks make use of multiple enzymes, it is important to know what has been digested with which, so the parts will fit together properly upon ligation.

Latest revision as of 19:53, 13 June 2008

Today

  • Developed the Westerns after an overnight exposure. Blank yet again. James thought the problem was due to the development solution used - it was an old tube in the fridge that had been mixed months ago and was probably no good anymore. New solution was made and applied, film was exposed for 60 seconds and again, there were no results. This is odd because there were obvious thick bands of overexpressed proteins when we did the Coomassie staining. We will need to set up some cultures when we use the Ni-NTA columns so perhaps we will do them in duplicate and use one set for Westerns again.
  • Digested I725021,I725022,I725025 and I725099 with xbal and pst
  • Did miniprep on Tom's 2 night+ 1 day "overnight", didn't get a high yeild of DNA, so tried to run them on a gel.
  • Got results back from Winnie's sequencing of the old Blue Ox biobrick. The sequences look good but they dont match the reference sequences at all. Dunno what's going on here but it probably doesn't matter because we are remaking all of the bricks anyway.

Lab Tip of the Day

When you do a digest, make sure you label the tubes clearly and be sure to include the name of the enzymes you used to do the digest. Since the BioBricks make use of multiple enzymes, it is important to know what has been digested with which, so the parts will fit together properly upon ligation.