Template:Kyoto/Notebook/Sep 1

(Difference between revisions)

Revision as of 00:44, 23 September 2013

No name

Name	Sample	Competent Cells	Total	Plate
8/31 tRNA-Spinach(pSB1C3)	2µL	20µL	22µL	CP
8/31 pT181 antisense(pSB1C3)	2µL	20µL	22µL	CP
8/31 pT181 attenuator(pSB1C3)	2µL	20µL	22µL	CP
8/31 pT181 antisense(pSB1C3)	2µL	20µL	22µL	CP
8/31 pT181 attenuator(2)-DT	2µL	20µL	22µL	CP
8/31 pT181 antisense-DT	2µL	20µL	22µL	CP
8/31 tRNA-Spniach-DT	2µL	20µL	22µL	CP
8/31 RBS-lysis2-DT	2µL	20µL	22µL	CP
8/31 Pconst-RBS-tetR-DT	2µL	20µL	22µL	Amp
8/31 Plac-RBS-lacZα-DT	2µL	20µL	22µL	CP
8/31 Ptet-RBS-lacZα-DT	2µL	20µL	22µL	CP
8/31	2µL	20µL	22µL	CP

No name

PreDenature	Denature	Annealing	Extension	cycle
94°C	94°C	55°C	68°C	--
5min	30s	30s	30min	30cycle

Nakamoto

state	Vector		Inserter		Ligation High ver.2
experiment	DT(E+S)	5.5	8/28 RBS-lysis1(E+S)2.4ng/µL	2.4

1. Samples were evaporeted used evaporator into about 7 µL. 2. Add Ligation High 3.5&micro:L and incubate 16&dig:C 1hour.

No name 5xM9 liquid medium

1. mix 5xM9 medium and 3.75%Agar solution 400mL
2. Add 1M MgSO4, 2M Glucose and 1 VitaminB1 0.5mL
3. Add CaCl2 while shaking Erlenmeyer flask.

@@ Line 64: / Line 64: @@
 </div>
 ===Ligation===
+<div class="experiment">
+<span class="author">Nakamoto</span>
+{| class="wikitable"
+!state||colspan="2"|Vector||colspan="2"|Inserter||Ligation High ver.2
+|-
+|experiment||DT(E+S)||5.5||8/28 RBS-lysis1(E+S)2.4ng/&micro;L||2.4
+|}
+. Samples were evaporeted used evaporator into about 7 µL.
+. Add Ligation High 3.5&micro:L and incubate 16&dig:C 1hour.
+</div>
 ===Liquid Culture===