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Construction of a set of Saccharomyces cerevisiae vectors designed for recombinational cloning Vincent Van Mullem, Maxime Wery, Xavier De Bolle, and Jean Vandenhaute

Yeast (2003) 20, 739 - 740

The Gateway technology allows the transfer of any ORF flanked by specific recombination sites into any vectors harbouring the corresponding sites. These 20 Saccharomyces cerevisiae Gateway compatible vectors are designed for expression without tag sequence or for C- or N-terminal protein tagging with 3HA (haemagglutinin), 13myc, 4TAP (tandem affinity purification) or GST (glutathione S-transferase) epitopes. The centromeric vectors allow expression of DNA sequence in yeast under tetracycline-regulatable promoters, while expression from the high copy vectors is driven by PGK promoter. 

accession no.	plasmid name	description
P30205	pVV200	TRP1, 2 um
P30206	pVV201	3HA, TRP1, 2 um
P30207	pVV202	GST, TRP1, 2 um
P30208	pVV203	13myc, TRP1, 2 um
P30209	pVV204	TRP1, CEN
P30210	pVV205	3HA, TRP1, CEN
P30211	pVV206	GST, TRP1, CEN
P30212	pVV207	13myc, TRP1, CEN
P30213	pVV208	URA3, CEN
P30214	pVV209	3HA, URA3, CEN
P30215	pVV210	GST, URA3, CEN
P30216	pVV211	13myc, URA3, CEN
P30217	pVV214	URA3, 2 um
P30218	pVV215	3HA, URA3, 2 um
P30219	pVV216	GST, URA3, 2 um
P30220	pVV217	13myc, URA3, 2 um
P30221	pVV220	4TAP, TRP1, 2 um
P30222	pVV221	4TAP, TRP1, CEN
P30223	pVV222	4TAP, URA3, CEN
P30224	pVV223	4TAP, URA3, 2 um



  8-Feb-2008
Matthias Rose

SGD