Team:BYU Provo/Team Thermosensor/Week11

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Latest revision as of 08:26, 24 September 2011

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Week 11 (June 26 - Jul 2)

6/27/11

It looks like 33-1 worked, but I don’t know if lacZ and GFP were actually inserted

Doesn’t look like lacZ did, but GFP looks promising.

6/28/11

PCR purfication of 33-1 (lacZ PCR)

Qiaquick PCR purification kit protocol -Julie

lacZ restricition digest (TRD 34-1)

T33-1 PCR up/lacZ with 1 ul of HindIII and XbaI each

pPLAT-Bad restriciton digest (TRD 34-2)

pIG 13 with 1 ul each of HindIII and XbaI

Ran a low melt. Cut out pPLAT-Bad and stuck in 1.5 centrifuge tube. Could not see lacZ band...->doesn’t matter, I used wrong lacZ reverse

We could run another low melt and we may want to PCR it again. Other half of low melt in fridge.

lacZ PCR (35-1)

Phusion polymerase and 1 ul each of IG40 and IG41 primers with pIGGY template
Making two in case there is another purification problem or something

35-2: PCR up of lacZ according to qiaquick instructions

6/30/11

Running gel on lacZ PCR products

Both lanes look good. Now onto restriction digest.

RD lacZ (35-3)

1-2 ul each restricition enzyme (HindIII and XbaI)

35-4 Ran low melt and cut out lacZ band. Very faint, but there!

lacZ/pPlatbad ligation 36-1

T4 ligase, 3 ul vector, 3 ul lacZ (added a little extra b/c faintness of band)

7/1/11

lacZ/pPlatbad transformation

Followed Grose protocol

Plated 100 ul on LB-amp and incubated overnight

Labeled T36-1 lacZ trans 1 July 2011 - Devin

@@ Line 11: / Line 11: @@
 <div id='pageContents'>
+==Week 11 (June 26 - Jul 2)==
+===6/27/11===
+It looks like 33-1 worked, but I don’t know if lacZ and GFP were actually inserted
+Doesn’t look like lacZ did, but GFP looks promising.
+===6/28/11===
+PCR purfication of 33-1 (lacZ PCR)
+* Qiaquick PCR purification kit protocol -Julie
+lacZ restricition digest (TRD 34-1)
+* T33-1 PCR up/lacZ with 1 ul of HindIII and XbaI each
+pPLAT-Bad restriciton digest (TRD 34-2)
+* pIG 13 with 1 ul each of HindIII and XbaI
+Ran a low melt. Cut out pPLAT-Bad and stuck in 1.5 centrifuge tube. Could not see lacZ band...->doesn’t matter, I used wrong lacZ reverse
+We could run another low melt and we may want to PCR it again. Other half of low melt in fridge.
+lacZ PCR (35-1)
+* Phusion polymerase and 1 ul each of IG40 and IG41 primers with pIGGY template
+* Making two in case there is another purification problem or something
+-2: PCR up of lacZ according to qiaquick instructions
+===6/30/11===
+Running gel on lacZ PCR products
+* Both lanes look good. Now onto restriction digest.
+RD lacZ (35-3)
+* 1-2 ul each restricition enzyme (HindIII and XbaI)
+-4 Ran low melt and cut out lacZ band. Very faint, but there!
+lacZ/pPlatbad ligation 36-1
+* T4 ligase, 3 ul vector, 3 ul lacZ (added a little extra b/c faintness of band)
+===7/1/11===
+lacZ/pPlatbad transformation
+Followed Grose protocol
+Plated 100 ul on LB-amp and incubated overnight
+Labeled T36-1 lacZ trans 1 July 2011 - Devin
 </div>