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Revision as of 09:59, 29 August 2010 (view source) Watachin (Talk | contribs) (New page: {{:Team:Tokyo_Metropolitan/Header}} ==2010/8/17 Tuesday (watachin)== ===Experiment:Electrophoreses of PCR productions=== '''Member'''<br /> NEX and watachin '''Materials''' *pSB1A3(25ng/...) ← Older edit		Revision as of 10:11, 29 August 2010 (view source) Watachin (Talk | contribs) Newer edit →
Line 20:		Line 20:
	'''Resalt'''		'''Resalt'''
		+
		+	[[Image:2010-08-17-ef.jpg]]
		+
		+	failure
		+
		+	Plasmid concentration was too low.
		+
		+	===Experiment:Transformation of pSB1A3===
		+	'''Member'''<br />
		+	NEX and watachin
		+
		+	'''Material'''
		+	*pSB1A3 1μl
		+	*competent cell DH5α 50μl
		+	*LB + amp plate
		+
		+	'''Procedure'''
		+	#mix pSB1A3 and DH5α
		+	#on ice (30min)
		+	#heat shock 42℃ 45sec
		+	#on ice (2min)
		+	#inoculate this onto plate
		+	#incubate cells at 37℃

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Revision as of 10:11, 29 August 2010

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2010/8/17 Tuesday (watachin)

Experiment:Electrophoreses of PCR productions

Member
NEX and watachin

Materials

• pSB1A3(25ng/μl) 22μl
• 10*Loading buffer 2.2μl
• DNA Marker 5μl
• 1*TAE buffer
• 1% agarose gel

Procedure

1. set agarose gel and add TAE buffer in gel box.
2. mix Loading Buffer and pSB1C3 and then put in well them(marker sets another well).
3. load DNA at 100V for two third of entire (about 15 minutes).
4. image the consequence of electrophoreses.

Resalt

failure

Plasmid concentration was too low.

Experiment:Transformation of pSB1A3

Member
NEX and watachin

Material

• pSB1A3 1μl
• competent cell DH5α 50μl
• LB + amp plate

Procedure

1. mix pSB1A3 and DH5α
2. on ice (30min)
3. heat shock 42℃ 45sec
4. on ice (2min)
5. inoculate this onto plate
6. incubate cells at 37℃