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Revision as of 01:24, 26 September 2012 (view source) Ryankenny (Talk | contribs) ← Older edit		Latest revision as of 01:24, 26 September 2012 (view source) Ryankenny (Talk | contribs)
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	<center><h1>Restriction Digest</h1></center>		<center><h1>Restriction Digest</h1></center>
-	<p>We prepared Master Mixes containing to following volumes,</p>	+	<p>We prepared Master Mixes containing the following volumes,</p>
	<center><table><tr><td><table border="3" cellpadding="4" cellspacing="0">		<center><table><tr><td><table border="3" cellpadding="4" cellspacing="0">
	<tr><td colspan="2">EcoR1 + Spe1 Master Mix</td></tr>		<tr><td colspan="2">EcoR1 + Spe1 Master Mix</td></tr>

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Latest revision as of 01:24, 26 September 2012

Restriction Digest

We prepared Master Mixes containing the following volumes,

EcoR1 + Spe1 Master Mix Substrate Volume (µL) 10x Buffer 20 EcoR1 2.5 Spe1 2.5 Water 75 Total 100

Xba1 + Pst Master Mix Substrate Volume (µL) 10x Buffer 20 Xba1 2.5 Pst 2.5 Water 75 Total 100

EcoR1 + Pst Master Mix Substrate Volume (µL) 10x Buffer 20 EcoR1 2.5 Pst 2.5 Water 75 Total 100

Protocol

1. Mix 10 µL of the desired DNA/plasmid and 10 µL of the appropriate Master Mix in a PCR tube.
2. Using a thermocycler, incubate the mixture at 37°C for 30 minutes and then deactivate the enzymes by heating to 80°C for 20 minutes.
3. Store in a -20°C freezer until DNA required