Revision as of 23:21, 19 July 2008

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Things we did today

Margaret

Margaret

Grace

Gel OK this time (95V for 50 min; ladder resolved, loading dye didn't run funny)
Incorrect bands still for B0015, J04430, R0010; Krystle will redo the plasmid preps for these
Correct bands for GFP fusion and BB-pRL1383a. BB-pRL1383a band faint -- why?

**DNA concentrations of PCR products**
PCR Sample	Concentration (1st measurement)	Concentration (2nd measurement)
nir	1015 ng/μl	1010 ng/μl
slr2016-1	1295 ng/μl	1107 ng/μl
slr2016-2	1518 ng/μl	1266 ng/μl
pilA	1312 ng/μl	1330 ng/μl
B0024	1546 ng/μl	1474 ng/μl
B0034	1537 ng/μl	1386 ng/μl
C0012	2130 ng/μl	1530 ng/μl
E0040	1502 ng/μl	1236 ng/μl
J33207	1454 ng/μl	1223 ng/μl
BB-pRL1383a	2279 ng/μl	2129 ng/μl
GFP fusion	1660 ng/μl	1714 ng/μl

Margaret, Krystle (thanks for the help!)

Grace, Krystle, Margaret

History is the only laboratory we have in which to test the consequences of thought. - Étienne Gilson

[http://manoa.hawaii.edu/ ][http://manoa.hawaii.edu/ovcrge/ ][http://www.ctahr.hawaii.edu ]

@@ Line 11: / Line 11: @@
 ===Extraction of Biobricks and Transformation in DB3.1===
 :<strong>Margaret</strong>
-:*streaked plates on Amp100 plates, but they took a long time to dry, so left in hood. The only problem is I came back later and the light was on... but for how long? (Just a reminder in case I get lawns everywhere. If this happens, just replica plate it???)
+:*streaked plates on Amp100 plates
 :*for details please look [[Team:Hawaii/Initial E. Coli Transformation|here]].
@@ Line 71: / Line 71: @@
 == Drylab Work ==
-===pRL1383a paper===
-<strong>Margaret</strong>
-:*Continued to work on my paper.(Another reminder... keep doing this!)
 ===[[Team:Hawaii/Project|Project Description (Abstract]])===