Method for Cloning Restriction Fragments Containing the Termini of BAC Inserts | Zendy

Tammy R. Plyler | Zendy; C. Eduardo Vallejos | Zendy

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Method for Cloning Restriction Fragments Containing the Termini of BAC Inserts

Author(s) -

Tammy R. Plyler,

C. Eduardo Vallejos

Publication year - 2000

Publication title -

biotechniques

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.617

H-Index - 131

eISSN - 1940-9818

pISSN - 0736-6205

DOI - 10.2144/00285rr07

Subject(s) - cloning (programming) , restriction enzyme , biology , genetics , molecular cloning , computational biology , restriction fragment , restriction map , restriction site , microbiology and biotechnology , base sequence , dna , gene , computer science , peptide sequence , programming language

We have developed a method to isolate the termini of BAC clones. The method is based on the two unique NotI sites located approximately 300 bp on either side of the EcoRI cloning site of the BAC vector pECSBAC4. Our strategy includes the following steps: (i) generation of Southern blots with BAC clones digested with NotI and a second restriction enzyme; (ii) identification of the termini attached to the NotI/EcoRI fragment of the BAC vector via hybridization with a probe derived from sequences located between one NotI site (left or right arm) and the cloning site; (iii) ligation of the doubly digested BAC clone (NotI and the selected second restriction enzyme) with an equally doubly digested cloning plasmid vector; and (iv) confirmation of the clone as a terminus. This strategy has allowed us to begin the construction of a contig near a common bean gene that controls resistance to a group of potyviruses.

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