From 2007.igem.org

< Melbourne | Lab BL Notebook(Difference between revisions)

Latest revision as of 15:15, 10 October 2007

Protocol for PCR reactions A~G

For amplifying the photoreceptor and transmembrane domains of NpSopII-NpHtrII.

PCR mix

PCR program

PrimerII

5ul 10x buffer\\

5ul Enhancer

0.6ul dNTPs (25mM stock)

2.5ul MgSO4 (Supplied in PCR kit)

1.5ul Primer BL_FP1_s (10uM stock)

1.5ul Primer II (10uM stock)

1ul Template (pJS010)

0.4ul Pfx Platinum (Invitrogen)

32.5ul ddH₂O

94°C - 5'

94°C - 30"

59°C - 35"

68°C - 1.5' (goto step 2 x30)

68°C -10'

4°C forever

Reaction A => Primer BL_Con1_as

Reaction B => Primer BL_Con2_as

Reaction C => Primer BL_Con3_as

Reaction D => Primer BL_Con4_as

Reaction E => Primer BL_Con5_as

Reaction F => Primer BL_Con6_as

Reaction G => Primer BL_Con7_as

50ul Total

Protocol for PCR reactions 1-7

For amplification of the kinase domain of ComP

PCR mix

PCR program

PrimerI

5ul 10x buffer\\

0.6ul dNTPs (25mM stock)

2.5ul MgSO4 (Supplied in PCR kit)

1.5ul Primer I (10uM stock)

1.5ul Primer VR (10uM stock)

1ul Template (pJS010)

0.4ul Pfx Platinum (Invitrogen)

32.5ul ddH₂O

94°C - 5'

94°C - 30"

59°C - 35"

68°C - 1.5' (goto step 2 x30)

68°C - 10'

4°C forever

Reaction A => Primer BL_Con1_s

Reaction B => Primer BL_Con2_s

Reaction C => Primer BL_Con3_s

Reaction D => Primer BL_Con4_s

Reaction E => Primer BL_Con5_s

Reaction F => Primer BL_Con6_s

Reaction G => Primer BL_Con7_s

50ul Total

@@ Line 1: / Line 1: @@
-=Protocol for PCR reactions A~G= (and -ve control) amplifying the photoreceptor and transmembrane domains of NpSopII-NpHtrII.
+=Protocol for PCR reactions A~G=
+For amplifying the photoreceptor and transmembrane domains of NpSopII-NpHtrII.
-====PCR mix====
+{| border="2" cellpadding="4" cellspacing="0" style="margin: 1em 1em 1em 0; background: #f9f9f9; border: 1px #aaa solid; border-collapse: collapse;"
-*5ul 10x buffer
+|-
-*5ul Enhancer
+! PCR mix
-*0.6ul dNTPs (25mM stock)
+! PCR program
-*2.5ul MgSO4 (Supplied in PCR kit)
+! [[Melbourne/Lab_BL_Notebook/PrimersI|PrimerII]]
-*1.5ul Primer I (10uM)
+|-
-*1.5ul Primer II (10uM)
+|5ul 10x buffer\\
-*1ul Template ([[Melbourne/pJS010|pJS010]])
-*0.4ul Pfx Platinum (Invitrogen)
-*32.5ul ddH<sub>2</sub>O
-----
+ul Enhancer
-ul Total
+.6ul dNTPs (25mM stock)
+.5ul MgSO4 (Supplied in PCR kit)
+.5ul Primer [[Melbourne/Lab_BL_Notebook/PrimersI#Oligo_15|BL_FP1_s]] (10uM stock)
+.5ul Primer II (10uM stock)
+ul Template ([[Melbourne/pJS010|pJS010]])
+.4ul Pfx Platinum (Invitrogen)
+.5ul ddH<sub>2</sub>O
+|94°C -  5'
+°C  - 30"
+°C  - 35"
+°C  - 1.5' (goto step 2 x30)
+°C  -10'
+°C forever
+|Reaction A => Primer BL_Con1_as
+Reaction B => Primer BL_Con2_as
+Reaction C => Primer BL_Con3_as
+Reaction D => Primer BL_Con4_as
+Reaction E => Primer BL_Con5_as
+Reaction F => Primer BL_Con6_as
+Reaction G => Primer BL_Con7_as
+|-
+| 50ul Total
+|}
+=Protocol for PCR reactions 1-7=
+For amplification of the kinase domain of ComP
+{| border="2" cellpadding="4" cellspacing="0" style="margin: 1em 1em 1em 0; background: #f9f9f9; border: 1px #aaa solid; border-collapse: collapse;"
+|-
+! PCR mix
+! PCR program
+! [[Melbourne/Lab_BL_Notebook/PrimersI|PrimerI]]
+|-
+|5ul 10x buffer\\
+.6ul dNTPs (25mM stock)
+.5ul MgSO4 (Supplied in PCR kit)
+.5ul Primer I (10uM stock)
+.5ul Primer VR (10uM stock)
+ul Template ([[Melbourne/pJS010|pJS010]])
+.4ul Pfx Platinum (Invitrogen)
+.5ul ddH<sub>2</sub>O
+|94°C -  5'
+°C  - 30"
+°C  - 35"
+°C  - 1.5' (goto step 2 x30)
+°C  - 10'
+°C forever
+|Reaction A => Primer BL_Con1_s
+Reaction B => Primer BL_Con2_s
+Reaction C => Primer BL_Con3_s
+Reaction D => Primer BL_Con4_s
+Reaction E => Primer BL_Con5_s
+Reaction F => Primer BL_Con6_s
+Reaction G => Primer BL_Con7_s
+|-
+| 50ul Total
+|}

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Melbourne/Lab BL Notebook/PCR1

From 2007.igem.org

Latest revision as of 15:15, 10 October 2007

Protocol for PCR reactions A~G

Protocol for PCR reactions 1-7