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From 2009.igem.org

Revision as of 09:49, 11 August 2009 (view source) Unocchi (Talk | contribs) ← Older edit		Revision as of 10:24, 11 August 2009 (view source) Unocchi (Talk | contribs) Newer edit →
Line 1:		Line 1:
-	コロニー数カウント(8/10にトラフォ行ったもの)	+	1.<B>Min prep</b><br>
-	No.   コロニー数	+	Checked the cell cultures transformed and plated out yesterday (8/10) for colony formation and made an approximate count of the number of colonies.
		+
		+	(plate number)-(location on plate) (no. of colonies)
	1-23L    100>		1-23L    100>
	1-15N    10		1-15N    10
Line 8:		Line 10:
	1-18C    10<		1-18C    10<
	1-20F    ×		1-20F    ×
-	液培(5mL)にAmp 5uL , Kan 25uL入れて植菌	+
		+	inoculate to iquid medium(5mL + Amp 5uL or Kan 25uL)
		+
		+	2.<B>digestion and ligation</b><br>
-	制限酵素処理	+	digestion with restriction enzyme
-	Vector	+	Vector1
	1-2M  12		1-2M  12
	SpeⅠ 1		SpeⅠ 1
Line 20:		Line 25:
	total 20uL		total 20uL
-	Insert	+	Insert1
	2-8M  5		2-8M  5
	XbaⅠ  1		XbaⅠ  1
Line 29:		Line 34:
-	Vector	+	Vector2
	1-23L  12		1-23L  12
	EcoRⅠ 1		EcoRⅠ 1
Line 37:		Line 42:
	total  20uL		total  20uL
-	Insert	+	Insert2
	3-18O  5		3-18O  5
	EcoⅠ  1		EcoⅠ  1
Line 45:		Line 50:
	total  20uL		total  20uL
-	2時間ほど37℃で反応させた	+	↓
		+	37℃ , 2hr
-		+	↓<br>
-	電気泳動	+	gel electrophoresis<br>
-	ゲル切り出し	+	gel cut<br>
-	精製を経て	+	↓<br>
-		+	purification by [QIAquick Nucleotide Removal Kit]<br>
-	ライゲーション	+	↓<br>
-	それぞれ	+	ligation
-	DNA溶液    44	+	ligation
		+	DNA        44
	10* buffer 5		10* buffer 5
-	ライゲース 1	+	ligation  1
	total      50uL		total      50uL
		+	↓
		+	16℃ overnight
-	トランスフォーメーション	+	3.<B>Transformation</b><br>
-	各2uL , 1-14F は 4uL	+	to get new plasmid
		+	each 4uL(DNA) , 1-14F : 2uL
	1-14H kan		1-14H kan
	1-14F kan		1-14F kan
-	2-18F Amp ('8/10コンピ	+	2-18F Amp ('8/10competent cell
	1-23J Amp		1-23J Amp
-	1-12C Amp (スーパーコンピ	+	1-12C Amp (super competent cell??
-		+
-	KanのものはLB培地を加えた後、小さな試験管に入れて振とう培養(1~2hr)してからプレートにまいた	+

---

Revision as of 10:24, 11 August 2009

1.Min prep
Checked the cell cultures transformed and plated out yesterday (8/10) for colony formation and made an approximate count of the number of colonies.

(plate number)-(location on plate) (no. of colonies)
1-23L    100>
1-15N    10
2-6P     10<
1-6I     10<
1-12H    10
1-18C    10<
1-20F    ×

inoculate to iquid medium(5mL + Amp 5uL or Kan 25uL)

2.digestion and ligation

digestion with restriction enzyme

Vector1
1-2M  12
SpeⅠ 1
PstⅠ 1
No.2 Buffer 2
dH2O 4
total 20uL

Insert1
2-8M   5
XbaⅠ  1
PstⅠ  1
No.2   2
dH2O   11
total  20 uL


Vector2
1-23L  12
EcoRⅠ 1
XbaⅠ  1
No.2   2
dH2O   4
total  20uL

Insert2
3-18O  5
EcoⅠ  1
SpeⅠ  1
No.2   2
dH2O   11
total  20uL

↓
37℃ , 2hr

↓
gel electrophoresis
gel cut
↓
purification by [QIAquick Nucleotide Removal Kit]
↓
ligation

ligation
DNA        44
10* buffer 5
ligation   1
total      50uL
↓
16℃ overnight

3.Transformation
to get new plasmid

each 4uL(DNA) , 1-14F : 2uL
1-14H kan
1-14F kan
2-18F Amp ('8/10competent cell

1-23J Amp
1-12C Amp (super competent cell??

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