Home Feedback Search Online Order CATALOG

International 

+32 (0) 16 58 90 45

+32 (0) 16 50 90 45

France

01 43 25 01 50

01 43 25 01 60

Italy

02 36 00 65 93

02 36 00 65 94

Germany

0241 6085 13140

0241 6085 33033
Back Up Next


 

 

shRNAmir Design

Expression Arrest shRNAmir triggers have been designed to mimic a natural microRNA primary transcript and each target sequence has been selected based on thermodynamic criteria for optimal small RNA performance. Validation of this design is detailed in Silva et al (2005) showing a substantial increase in knockdown efficiency.

Advantages of shRNAmir design

  • Replaced mature microRNA sequence in mir-30 with gene specific duplexes
  • Adding mir-30 loop and context sequences adds endogenous processing by Drosha which increases subsequent Dicer recognition and specificity
  • Dicer processing promotes active loading into the RISC complex
  • Rules based design include destabilizing the 5"end of the antisense strand for strand specific incorporation into RISC

Increased Drosha/Dicer processing=More siRNA=Greater knockdown


 
shRNAmir produce increased knockdown

 

shRNAmir constructs produce greater and more consistent knockdown of target genes when compared against conventionally designed shRNA to the same genes. Multiple shRNAs againstvarious proteasomal genes were tested in a functional assay and the data averaged.

 

 
References:
  1. Paddison, P et al (2004) 'Cloning of short hairpin RNAs for gene knockdown in mammalian cells' Nature Methods Vol 1:2, 163-167
  2. Silva, J et al (2005) 'Second-generation shRNA libraries covering the human and mouse genomes' Nature Genetics Vol 37:11, 1281-88.
  3. Lee, Y et al (2002) ‘MicroRNA maturation: stepwise processing and subcellular localization' EMBO Vol 21, 17: 4663-4670.
  4. Chendrimada et al (2005) 'TBRP recruits the Dicer complex to Ago2 for microRNA processing and gene silencing' Nature Vol 436, 740-744.
  5. Gregory et al (2005) 'Human RISC couples microRNA biogenesis and post-transcriptional gene silencing' Cell, Vol 123, 631-640.

 

Unique microRNA adapted design
 

shRNAmir produce 12 fold greater processed siRNA
 

Northern blotting was used to detect the mature siRNA produced after transfection of Hek 293 cells with shRNA or shRNAmir. 12 fold greater siRNA was detected after shRNAmir processing vs shRNA processing (from Silva et al 2005)
Purchasing Information
Catalog No.
Description
Literature
Buy
RHS1764
Human retroviral shRNAmir individual clone
 
RHS4430
Human GIPZ lentiviral shRNAmir individual clone 
 
RMM1766
Mouse retroviral shRNAmir individual Clone 
 

 

 

For more information :: Bioxys and Gentaur BVBA :: Av. de l'Armée 68 B4 :: BE-1040 BELGIUM

Email: info@gentaur.com
 

International 

+32 (0) 16 58 90 45

+32 (0) 16 50 90 45

France

01 43 25 01 50

01 43 25 01 60

Italy

02 36 00 65 93

02 36 00 65 94

Germany

0241 6085 13140

0241 6085 33033
Send mail to webmaster with questions or comments about this web site.
Copyright © 2005 Gentaur BVBA
Last modified: feb-07