Team:UESTC-China/Protocol

DNA ligation with T4 DNA Ligase

Component	20ul Reaction
1.33X Master Mix	15ul
Insert DNA	the moles of insert DNA to vector DNA is 5：1
>Vector DNA	50ng
ddH2O	To 20ul
Incubate at 50℃ for 1 hour

DNA ligation with Gibson Assemble

Component	20ul Reaction
Vector DNA	50ng
Insert DNA	the moles of insert DNA to vector DNA is 5：1
10X T4 DNA ligase buffer	2ul
T4 DNA ligase	1ul
ddH2O	to 20ul
Incubate at 25℃ for 12 hours

Double Digestion of DNA

Component	50ul Reaction
10x FastDigest buffer	5ul
Restriction enzyme 1	1ul
Restriction enzyme 2	1ul
DNA	1-2ug
ddH2O	to 50ul
Incubate at 37℃ for 2 hours

PCR protocol for KOD-Plus-Neo

Component	50ul Reaction
ddH2O	33ul
10X buffer for KOD-Plus-Neo	5ul
MgSO4	1ul
10mM dNTPs	1ug
10uM forward primer	1ul
10uM reverse primer	1ul
Template	1ul
KOD enzyme	1ul

	Temperature	Time	Cycle
Step1	94℃	30s	X35 cycles
	56℃	30s
	68℃	30s/kb
Step3	68℃	5min	X1 cycles
	10℃	10min
10uM reverse primer	1ul	ddH2O	33ul

PCR protocol for KOD-Plus-Neo

Component	50ul Reaction
ddH2O	32ul
10X buffer for KOD-Plus-Neo	5ul
MgSO4	3ul
10mM dNTPs	5ul
10uM forward primer	1ul
10uM reverse primer	1ul
Template	1ul
KOD enzyme	1ul
Each template will be diluted by the number of moles into 2-10ng/ul.

	Temperature	Time	Cycle
Step1	94℃	5min	X1 cycle
Step2	94℃	30s	X35 cycles
	56℃	30s
	68℃	30s/kb
Step3	68℃	5min	X1 cycles
	10℃	10min

Colony PCR with Taq DNA polymerase

Component	25ul Reaction
ddH2O	15.8ul
10X Taq buffer	2.5ul
2.mM dNTPs	0.5ul
10uM forward primer	0.5ul
10uM reverse primer	0.5ul
Taq enzyme	0.2ul
Water with colony	5ul

	Temperature	Time	Cycle
Step1	95℃	5min	X1 cycles
Step2	94℃	30s	X35 cycles
	56℃	30s
	72℃	1min/kb
Step3	72℃	10min	X1 cycles
	10℃	10min