"

 

From 2009.igem.org

Revision as of 07:50, 3 October 2009 (view source) Kaoru Yamamoto (Talk | contribs) (→PCR) ← Older edit		Latest revision as of 08:00, 3 October 2009 (view source) Kaoru Yamamoto (Talk | contribs) (→Digestion Test)
Line 35:		Line 35:
	*Sample		*Sample
	Vector(plux-GFP)		Vector(plux-GFP)
		+
		+	Insert(sfGFP)
		+
		+
		+	*Vector
		+	<table width="100" border="1" cellpadding="0"  cellspacing="0" bordercolor="#000000"><tr>
		+	<td width="50">Vector DNA</td>
		+	<td width="50">30 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>Nco1</td>
		+	<td>1 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>BamH1</td>
		+	<td>1 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>Buffer3</td>
		+	<td>5 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>BSA</td>
		+	<td>5 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>NFW</td>
		+	<td>8 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>Total</td>
		+	<td>50 &mu;L</td>
		+	</tr>
		+	</table>
		+
		+
		+
		+	*Insert
		+	<table width="100" border="1" cellpadding="0"  cellspacing="0" bordercolor="#000000"><tr>
		+	<td width="50">Insert DNA</td>
		+	<td width="50">20 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>Nco1</td>
		+	<td>1 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>BamH1</td>
		+	<td>1 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>Buffer3</td>
		+	<td>3 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>BSA</td>
		+	<td>3 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>NFW</td>
		+	<td>2 &mu;L</td>
		+	</tr>
		+	<tr>
		+	<td>Total</td>
		+	<td>30 &mu;L</td>
		+	</tr>
		+	</table>
		+
Line 45:		Line 113:
	Took a picture		Took a picture
-
-
-
	== Transformation ==		== Transformation ==

---

Latest revision as of 08:00, 3 October 2009

>Go to the Notebook page

(28_September_2009 <|>30_September_2009)

Contents 1 Gel electrophoresis 2 Digestion Test 3 Transformation 4 Digestion 5 PCR

Gel electrophoresis

Yesterday's oparation is here.

• Today's operation

10:40-

Mini Prep.

13:30-

Gel electrophoresis(135 V, 27 min)

---DNA Clean & Concentrator---

15:50-

Gel electrophoresis again(135 V, 27 min)

Digestion Test

• Sample

Vector(plux-GFP)

Insert(sfGFP)

• Vector

Vector DNA	30 μL
Nco1	1 μL
BamH1	1 μL
Buffer3	5 μL
BSA	5 μL
NFW	8 μL
Total	50 μL

• Insert

Insert DNA	20 μL
Nco1	1 μL
BamH1	1 μL
Buffer3	3 μL
BSA	3 μL
NFW	2 μL
Total	30 μL

18:55-

Gel electrophoresis(135 V, 25 min)

19:45

Took a picture

Transformation

• Sample

Competent Cells : XL10G(K)

Plasmid : plux-GFP(Cm)

21:45-

CmのプレートにまいてCultured it at 37 degrees Celsius.

Digestion

• Sample

Vector : plux-GFP(p15A)

Insert : sfGFP

Enzymes : Nco1, BamH1

21:17

We added Enzymes and took it 37 degrees Celsius.

---3 h---

We took it 65 degrees Celsius for 酵素を失活させる

---20 min---

24:42

We kept it in refrigerator.

PCR

• Template

plux-HSUTK

• Element of mixtures

Template	1 μL
Primer(F)	2.5 μL
Primer(R)	2.5 μL
Buffer(x 10)	5 μL
dNTP	4 μL
DNA pol.	1 μL
dH2O	34 μL
Total	50 μL

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