Methods for dynamic vector assembly of DNA cloning vector plasmids

摘要

A method for using cloning vector plasmids to produce DNA molecules, such as transgenes, in a single cloning step. The transgenes can be used for the purpose of gene expression or analysis of gene expression. The plasmid cloning vectors are engineered to minimize the amount of manipulation of DNA fragment components by the end user of the vectors and the methods for their use. Transgenes produced using the invention may be used in a single organism, or in a variety of organisms including bacteria, yeast, mice, and other eukaryotes with little or no further modification.

主权项

1. A method for simultaneously synthesizing an array of transgenes, comprising:
a. providing a primary cloning vector plasmid comprising a first and a second docking point,
wherein each docking point comprises at least one endonuclease site of greater than six nucleotides, andwherein the cloning vector plasmid further comprises a unique homing endonuclease site in a forward orientation located upstream from the 5′ end of the first docking point and a unique homing endonuclease site in a reverse orientation located downstream from the 3′ end of the second docking point; b. introducing at least one Promoter nucleotide sequence into a corresponding Promoter shuttle vector; c. introducing at least one Expression nucleotide sequence into a corresponding Expression shuttle vector; d. introducing at least one Regulatory nucleotide sequence into a corresponding Regulatory shuttle vector; e. simultaneously ligating the Promoter, Expression, and Regulatory nucleotide sequences from the Promoter, Expression, and Regulatory shuttle vectors to the cloning vector plasmid, between the first and second docking points, thereby forming a transgene construct comprising the Promoter, Expression, and Regulatory nucleotide sequences; f. digesting the cloning vector plasmid with homing endonucleases that recognize the unique homing endonuclease sites in (a), thereby releasing the transgene construct; g. providing a second cloning vector plasmid comprising the same unique homing endonuclease site in a forward orientation and the same unique homing endonuclease site in a reverse orientation as the first cloning vector plasmid; h. digesting the second cloning vector plasmid with the homing endonuclease used in (f); and i. ligating the transgene construct of (f) into the second cloning vector plasmid.