LIC Cloning (Ligation independent cloning)

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Revision as of 12:04, 30 May 2025 by ESO wikiadmin (talk | contribs) (Created page with " == Procedure == Design primers compatible for cloning in vector containing the LIC sequence (e.g. pDNR Dual LIC) and perform PCR. Separate 4 µl of PCR reaction via agarose gel electrophoresis to check PCR product. Many unspecific bands besides the desired one require gel separation of the PCR sample and extraction of the desired band. If necessary, 2-3 PCR reactions can be pooled to gain more material. Add 10x NEB2 Buffer to the PCR sample to reach 1x end concentration...")
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Procedure

Design primers compatible for cloning in vector containing the LIC sequence (e.g. pDNR Dual LIC) and perform PCR. Separate 4 µl of PCR reaction via agarose gel electrophoresis to check PCR product. Many unspecific bands besides the desired one require gel separation of the PCR sample and extraction of the desired band. If necessary, 2-3 PCR reactions can be pooled to gain more material. Add 10x NEB2 Buffer to the PCR sample to reach 1x end concentration and add 2 µl of DpnI enzyme. Incubate 4 h at 37°C and inactivate enzyme at 80°C for 10 min. Purify PCR product with Qiagen PCR purification Kit. Determine concentration of PCR product at Nanodrop and calculate molarity.

Molarity Calculation for LIC Cloning

The molar concentration of the PCR product is calculated as follows:

cmol=cPCR×109Nbp×650

(Equation 1)

Variables:

  • cmol = molar concentration [pmol/μL]
  • cPCR = PCR product concentration [ng/μL]
  • Nbp = PCR product length [bp]
  • 650 = average molecular weight per base pair [g/mol]

Example: For a 1500 bp PCR product at 50 ng/μL:

cmol=50×1091500×650=51,282 pmol/μL

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