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Revision as of 19:21, 19 July 2010 (view source) Tgjohnst (Talk | contribs) (New page: {{:Team:Brown/templates/header}} ==Monday, June 28 2010== ===Competent cells:=== Overnight culture (from Sunday night) Diluted 1:250 in 250 mL LB media Incubate (shaking) 37°C until ...) ← Older edit		Latest revision as of 19:26, 19 July 2010 (view source) Tgjohnst (Talk | contribs) (→Preparation of Agar Plates)
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	===Preparation of Agar Plates===		===Preparation of Agar Plates===
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	*10g tryptone		*10g tryptone

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Latest revision as of 19:26, 19 July 2010

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Monday, June 28 2010

Competent cells:

Overnight culture (from Sunday night)

Diluted 1:250 in 250 mL LB media

Incubate (shaking) 37°C until ~0.4 OD at 600 nm (3 to 4 hours).

• • Started at 10:50 AM

12:55 PM – Transformation of pGEM ligation product into XL1Blues.

Preparation of Agar Plates

Agar recipe – cook on hot plate

• 10g NaCl
• 10g tryptone
• 5g yeast extract
• 20g agar
• Deionized water to a final volume of 1L

1. Autoclave
2. Let cool down, add Ampicillin to 100 µl/ml; mix well. (Add 1 ml amp at 100 mg/ml stock to 1L to get final concentration of 100 µg/ml.)
3. Pour

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Received our L. lactis from Ireland. 50 µl pPTPi, MG1614, and pPTPi in MG1614 (can act as a control)

Grown in M17 broth with 0.5% glucose, 6 µg/mL tetracycline at 30°C.