Team:Michigan/Oil Sands

This team includes [[User:annlesn|Ann Lesnefsky]], [[User:rajabiab|Bryce Rajabian]], [[User:chillywings|Marcus Lehr]], [[User:Infekt|Alex Pyden]], Jeremy Golden, John Seong Kyu Yang and [[User:kilholee|Kilho Lee]].

[[Team:Michigan/Oil_Sands_August_September]]

[[Media:Ph7_biofilm_assay_results.xls|10/1/10 pH7 Biofilm Assay]]

 

 

 

 

==='''In the Lab'''===

 

[[Image:Oilsands01.png|middle|250px]]

 

 

 

 

 

 

 

 

==10/1/2010==

 

Moved broth cultures 37°C to 4°C -- 1:30pm (19-hr culture)

Prepared biofilm assay plate for all pH9 tests - following [[Media:Static+biofilm+quantification.pdf|Alex's biofilm assay protocol]]

[[image:9-30 plate template.jpg]]

**100 μL/well: 99 μL medium + 1 μL culture

Started 24-hr kinetic reading for pH9 plate -- ~midnight

 

 

 

== 10/3/10 ==

 

 

== 10/4/2010 ==

 

 

***Flu PCR- 29.8 ng/uL x 17 uL= 506.6 ng / 50 uL = 10.132 ng/uL

***pSB1AT3- 240.5 ng/uL x 5 uL= 1202.5 ng / 50 uL = 24.05 ng/uL

 

*4 uL Flu PCR x 10.132 ng/uL= 40.528 ng

 

 

 

 

 

 

 

 

It should be noted that two 200 uL aliquots of cells had to be thawed, and one was labeled "Thawed" and returned to the -80 C. Thawing should be avoided if possible.

 

 

 

 

 

Surprisingly, they seem to grow better at pH 9, at least in co-culture. As expected, the co-culture did better than pure cultures. This lends some support towards Alex's biofilm assay results, however, it should still be repeated. Also, plated a serial dilution of the pH 9 co-culture, at 10^-5, 10^-6, and 10^-7 dilutions to determine the conversion factor between OD600 and cell count. Made streak plates of all other cultures, pure cultures for stock, and pH 7 co-culture to determine if colonies could be distinguished. All cultures and plates were returned to the 30^oC incubator, without shaking.

 

 

Kevin removed the transformation plates which were placed back in the incubator to the 4^oC around 1 pm.