New E. coli Cloning Vector Using a Cellulase Gene (celA) as a Screening Marker
Author(s) -
Soo Jin Jang,
W J Park,
Sung-Kyun Chung,
Choon-Soo Jeong,
Do Kwan Chung
Publication year - 2001
Publication title -
biotechniques
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.617
H-Index - 131
eISSN - 1940-9818
pISSN - 0736-6205
DOI - 10.2144/01315st07
Subject(s) - cellulase , cloning vector , cloning (programming) , molecular cloning , ecori , recombinant dna , restriction enzyme , biology , multiple cloning site , microbiology and biotechnology , shuttle vector , plasmid , escherichia coli , gene , genetics , expression vector , vector (molecular biology) , biochemistry , cellulose , gene expression , computer science , programming language
The extracellular endoglucanase A gene of Clostridium thermocellum (celA) was used as a screening marker for E. coli cloning vector A 1.4-kb EcoRI fragment containing celA from pTvec/celA was isolated and cloned into a pUC18 deleting beta-galactosidase gene fragment. The constructed vectors, pCEL1, pCEL10, pCEL11, and pCEL20, have different multiple cloning sites within celA. If the cellulase, CelA, is inactivated by insertion of a foreign DNA fragment into multiple cloning sites, the recombinant transformants show no clear halos on an agar plate containing cellulose. This process overcomes the ambiguity of color screening in the X-gal/beta-galactosidase system, and over 90% of the recombinant transformants with no halos have foreign DNA inserts. Several E. coli strains were transformed successfully with pCEL series vectors regardless of mutation for alpha-complementation. Because E. coli strains do not have a cellulase gene, a vector using a cellulase gene screening marker can be used in any E. coli strain without limit. The new cloning system is very efficient, convenient, and cost effective.
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