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Metastasis inhibition by BRMS1 and miR-31 replacement therapy in claudin-low cell lines

Iranian Journal of Basic Medical Sciences. 2019; 
Samila Farokhimanesh , , Mehdi Forouzandeh Moghadam *, Marzieh Ebrahimi
Products/Services Used Details Operation
Gene Synthesis In order to recognize possible target genes of miR-31, TargetScan, miRanda, miRDB, and PicTar databases were used. In order to reach maximum levels of expressions, GenScript (Genscript Corporation Piscataway; NJ, USA) was used to optimize the BRMS1 gene sequence. Next, the optimized gene was cloned into pcDNA 6.2-GW/ EmGFPmiRneg (pc.neg) control plasmid (Invitrogen, Carlsbad, CA, USA) (pc.BRMS1) and pcDNA 6.2-GW/ EmGFPmiR-31 (pc.miR-31.BRMS1) through SalI and DraI restriction enzymes (Roche Applied Science; Castle Hill; NSW, Australia). The resulting chimeric vector causes (co-cistronic) co-expression of BRMS1in the position of EmGFP and miRNA-31 included in a murine miR-155 setting under human cytomegalovirus promoter. Sequencing was used to confirm the accuracy of each chimeric vector. Get A Quote

摘要

Objective(s): The growing trend of research demonstrates that dynamic expression of two metastasis repressor classes (metastasis suppressor genes and anti-metastatic miRNA) has a close relationship with tumor invasion and metastasis. Using different strategies, it was revealed that cellular levels of miR-31 and Breast cancer Metastasis Suppressor1 (BRMS1) protein, which are among the most significant modulators of metastasis, have a correlation with the cell’s capability for invading and metastasizing; cells containing higher levels of miR-31 or BRMS1 were less metastatic. This project was carried out to determine whether the combinations of miR-31 and BRMS1 genes are able to enhance the capability of repress... More

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