精品久久久久久,在线观看精品国产,久久不卡,久久就是精品,国产精品无码久久久久,亚洲日本一区二区三区高清在线,亚洲午夜精品一级在线

Distribution host: Escherichia coli HB101 (ATCC 33694)

Size (kb): 6.6999998092651370

DESCRIPTION OF VECTOR:
Intact vector size: 6.700
Type of vector: plasmid
Cloning sites:
Polylinker sites:
Construction: pUC19
Host range: Saccharomyces cerevisiae; Escherichia coli
Features (with orientation and position when available):
replicon: pMB1
marker(s): ampR, <-
restriction site: EcoRI, SmaI
gene disruption cassette: ura3::TRP1/kanR
restriction site: SmaI

Vector: pUT11 (plasmid)

Construction: pUC19

Marker(s):TRP1,ampR,kanR

Construct size (kb): 6.699999809265137

Features: gene disruption cassette: ura3::TRP1/kanR
marker(s): ampR
replicon: pMB1
restriction site: EcoRI, SmaI
restriction site: SmaI

YI-type (integrating) shuttle vector

host modification

marker swap vector URA3 --> TRP1

Restriction digests of the clone give the following sizes (kb): HindIII--4.6, 2.0; SmaI--3.8, 2.7.

To convert the host phenotype from URA3 to TRP1, transform with the SmaI digested vector and select for Trp+ transformants.

Some combinations of marker swap plasmids and target locus may result in relatively high reversion rates. In most but not all cases the frequencies of successful convertants are greater than 30%.

A marker swap vector designed to change the S. cerevisiae host phenotype by one-step gene disruption of the URA3 gene with the TRP1 and kanR markers.

When swapping markers on an episomal plasmid, appropriate phenotype may result from loss of the plasmid unless a second selectable or scorable marker is used to ensure plasmid maintenance.

Vector was constructed by replacing an internal StuI fragment of URA3 with a SmaI fragment containing the TRP1 and kanR coding sequences. TRP1 and URA3 are in the same orientation.

Temperature: 37.0°C

component of:ATCC 87561