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Mega primer-mediated molecular cloning strategy for chimaeragenesis and long DNA fragment insertion
Author(s) -
Hui Zhang,
Changjun Liu,
Hui Jiang,
Lu Zhou,
Wenying Li,
Lingyun Zhu,
Lei Wu,
Er Meng,
Dongyi Zhang
Publication year - 2017
Publication title -
bioscience reports
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.938
H-Index - 77
eISSN - 1573-4935
pISSN - 0144-8463
DOI - 10.1042/bsr20160608
Subject(s) - primer (cosmetics) , cloning (programming) , mega , cloning vector , molecular cloning , transformation (genetics) , plasmid , primer dimer , genetics , biology , dna , computational biology , microbiology and biotechnology , polymerase chain reaction , gene , chemistry , computer science , multiplex polymerase chain reaction , complementary dna , physics , organic chemistry , astronomy , programming language
Molecular cloning methods based on primer and overlap-extension PCR are widely used due to their simplicity, reliability, low cost and high efficiency. In this article, an efficient mega primer-mediated (MP) cloning strategy for chimaeragenesis and long DNA fragment insertion is presented. MP cloning is a seamless, restriction/ligation-independent method that requires only three steps: (i) the first PCR for mega primer generation; (ii) the second PCR for exponential amplification mediated by the mega primers and (iii) DpnI digestion and transformation. Most importantly, for chimaeragenesis, genes can be assembled and constructed into the plasmid vector in a single PCR step. By employing this strategy, we successfully inserted four DNA fragments (approximately 500 bp each) into the same vector simultaneously. In conclusion, the strategy proved to be a simple and efficient tool for seamless cloning.

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