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Trypanosoma cruzi CRISPR/Cas9 System Plasmid, CAS9/pTREX-n

详细技术说明
Applications This plasmid expresses the fusion gene CAS9-HA-2xNS-GFP (S. pyogenes Cas9 sequence with atwice-repeated sequence of the simian virus 40 nuclear localization signal andGFP) in the pTREX-n backbone. This vector is used for cloning a specific sgRNAby BamHI, to be co-expressed with Cas9 for genome editing in Trypanosoma cruzi. Trypanosomacruziis the agent of Chagas disease, which affects millions of people worldwide.Vaccines to prevent this disease are not available, and drug treatments are notcompletely effective. The study of the biology of this parasite through geneticapproaches will make possible the development of new preventive or treatmentoptions.
*Abstract

Reagent Description

 

Name:  CAS9/pTREX-n

Gene/insert name:  Fusion gene CAS9-HA-2xNLS-GFP

Fusion Tag(s):  Fusion gene Cas9-HA-2xNLS-GFP

Antibiotic Resistance:  Ampicillin

Grow in E. coli at 37 C:  DH5alpha; 37C

Selectable markers:  Neomycin (select with G418)

Cloning Site 5':  XbaI

Cloning Site 3':  HindIII

Insert Size:  4975 bp

Vector Backbone and Size:  pTREX-n, backbone size without insert: 6227bp

High or low copy:  High

Storage:  -20C

 

Gene/Insert Name: Fusion gene CAS9-HA-2xNLS-GFP

Insert Size (bp):  4975

Species: Synthetic; Streptococcus pyogenes

Fusion Proteins/Tags: Fusion gene Cas9-HA-2xNLS-GFP  N/A  

Vector Backbone and Size: pTREX-n, backbone size without insert: 6227bp

Cloning Site 5': XbaI

Cloning Site 3': HindIII

Antibiotic Resistance: Ampicillin 

High or Low Copy: High

Grow in Standard E. coli @ 37C: DH5alpha

Selectable Markers: Neomycin (select with G418) 

Storage Temperature: -20C 

References

 

LanderN, Li ZH, Niyogi S, Docampo R. CRISPR/Cas9-Induced Disruption of ParaflagellarRod Protein 1 and 2 Genes in Trypanosomacruzi Reveals Their Role in Flagellar Attachment. mBIO. 2015.6(4): e01012-15.

国家/地区
美国

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