Team:Chiba/Notebook/Calendar/30 September 2009

From 2009.igem.org

Revision as of 23:22, 21 October 2009 by Kaoru Yamamoto (Talk | contribs)

(diff) ← Older revision | Latest revision (diff) | Newer revision → (diff)

>Go to the Notebook page

(29_September_2009 <|>1_October_2009)

Transformation

Yesterday's operation is here.

Today's operation

10:30-

Culture at 37 degrees Celsius

20:00-

Mini Prep.

20:40-

Digestion Test

20:56-

At 37 degrees Celsius

21:45-

Gel electro...(135 V, 25 min)

PCR

Yesterday's operation is here.

11:15-

Gel electro...(135 V, 27 min)

12:10

Took a picture

Cloning

Digestion

Yesterday's operation is here.

12:37-

Gel electro...(100 V, 40 min)

13:20

into ethyl bromide

13:35

Took a picture and cut the gel.

Then we added 2 mL of ADB Buffer and kept it at 37 degrees Celsius.

DNA Clean & Concentrator

We 溶出ed 50 μL.

SAP処理

まぜ表

15:45-

インキュベート it at 37 degrees Celsius.

---30 min---

16:20

We transferred it at 65 degrees Celsius and 失活させた

---15 min---

DNA Clean & Concentrator

We 溶出ed 20 μL.

Gel electro...

17:32

Electro...

18:15

Took a picture

Ligation

18:30

@Room Temperture

21:30

Transformation

21:50

@37 degrees Celsius

23:10

Plating

Team:Chiba/Notebook/Calendar/30 September 2009

From 2009.igem.org

Contents

Transformation

PCR

Cloning

Digestion

DNA Clean & Concentrator

SAP処理

DNA Clean & Concentrator

Gel electro...

Ligation