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Revision as of 01:27, 8 October 2008 (view source) Graham (Talk | contribs) ← Older edit		Revision as of 01:48, 10 October 2008 (view source) Nbakshi2 (Talk | contribs) Newer edit →
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	* PCR PGK Promotor		* PCR PGK Promotor
	** Finnzymes Phusion High Fidelity DNA Polymerase		** Finnzymes Phusion High Fidelity DNA Polymerase
		+	*** F-530, 20V (2V/uL)
		+
		+	**FiLL out PCR TABLE
		+
		+
		+	== 18th September ==
		+	* Ran ___? reaction
		+	* Extracted DNA from gel from 8th September (PGK Terminator)
		+	*FILL TABLE
		+
		+
		+	== 19th September ==
		+	* Gel of PGK Promotor has no DNA present
		+
		+
		+	== 23rd September ==
		+	* PCR: Fus1 Downstream
		+	* Fill PCR TABLE
		+
		+
		+	== 24th September ==
		+	* Ran gel of Fus1 Downstream
		+	** Result: No DNA present on gel
		+
		+
		+	== 25th September ==
		+	* PCR: Fus1 Upstream
		+
		+
		+	== 1st October ==
		+	* PCR: Ste2
		+
		+
		+	== 8th October ==
		+	* PCR: PGK Terminator
		+	** Use DNA extracted from gel on 18th September
		+
		+	* Also extracted DNA from gel from 30th September
		+
		+
		+
		+
		+
		+
		+
	<!-- == Insert Date Here ==		<!-- == Insert Date Here ==

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Revision as of 01:48, 10 October 2008

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Contents 1 22nd July 2 24th July 3 22nd August 4 25th August 5 26th August 6 27th August 7 28th August 8 2nd September 9 3rd September 10 8th September 11 9th September 12 10th September 13 11th September 14 12th September 15 15th September 16 18th September 17 19th September 18 23rd September 19 24th September 20 25th September 21 1st October 22 8th October

22nd July

• Yeast obtained from Dr. Zhao

24th July

• Prepared liquid culture for DNA extraction
• Made 1M Tris. Cl pH 8.0
• Made 4M ammonium acetate

22nd August

• Attempted DNA extraction
  • Result: Failed
• Obtained more yeast from Dr. Zhao

25th August

• Prepared overnight culture for DNA extraction (3:27pm)

26th August

• Attempted DNA extraction
• Prepped overnight culture

27th August

• Performed PCR (FILL IN PCR TABLE)
• Prepped 3 overnight cultures

28th August

• Extracted DNA from 4 cultures
• Ran gel of PCR products (1.5%, 200V)
  • Result: No bands present

2nd September

• FILL IN PCR TABLE

3rd September

• Ran gel
  • Ladder lane 7
  • Sample 7 spilled
  • 1% agarose
    • Too high
  • 120V
    • Too low
  • 50 minutes

8th September

• FILL IN PCR TABLE
• Prepped 4 overnight cultures
  • Yeast dried out again

9th September

• Signs of life in 3 of the cultures
  • Wait until tomorrow
• Ran gel on PCR from 8th September
  • 150V, 50 minutes
  • No sign of DNA
• Ladder from Courtney

10th September

• Ran gel again
• Split culture
  • 150V, 50 minutes
  • 0.75% gel
  • Ladder from Courtney

11th September

• FILL IN PCR TABLE

12th September

• Isolated DNA from 8 cultures
• Ran gel
  • 1% agarose
  • 150V
  • 38 mins
    • Poor results

15th September

• PCR PGK Promotor
  • Finnzymes Phusion High Fidelity DNA Polymerase
    • F-530, 20V (2V/uL)

• • FiLL out PCR TABLE

18th September

• Ran ___? reaction
• Extracted DNA from gel from 8th September (PGK Terminator)
• FILL TABLE

19th September

• Gel of PGK Promotor has no DNA present

23rd September

• PCR: Fus1 Downstream
• Fill PCR TABLE

24th September

• Ran gel of Fus1 Downstream
  • Result: No DNA present on gel

25th September

• PCR: Fus1 Upstream

1st October

• PCR: Ste2

8th October

• PCR: PGK Terminator
  • Use DNA extracted from gel on 18th September

• Also extracted DNA from gel from 30th September

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