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首頁 /診斷試劑 /腫瘤標準品 /Fusion /AI-Edigene? BCR-ABL1 (E14-E2) Fusion with ABL1 p.T315I Plus

AI-Edigene? BCR-ABL1 (E14-E2) Fusion with ABL1 p.T315I Plus

CBP20227R

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Introduction 
Format RNA
Description

Presence of a BCR-ABL1 fusion gene is necessary for the pathogenesis of CML. In up to 95% of cases, a t(9;22) (q34;q11) translocation results in the BCR-ABL1 fusion gene (Faderl et al. 1999). This translocation results in the Philadephia chromosome. In rare CML cases lacking the traditional t(9;22) translocation, other translocations result in the creation of the BCR-ABL1 fusion gene, which sometimes involve multiple chromosomes.
ABL1 is a tyrosine kinase, and, in normal cells, it plays a role in cellular differentiation and regulation of the cell cycle. The BCR-ABL1 fusion gene creates a constitutively active tyrosine kinase, which leads to uncontrolled proliferation.

ABL1 T315I is a gatekeeper mutation that lies within the hinge region of the protein kinase domain of the Abl1 protein (PMID: 18794843). T315I has been demonstrated to occur as a secondary resistance mutation and results in increased kinase activity and transformation in the context of BCR-ABL1 in cell culture (PMID: 11423618, PMID: 18794843, PMID: 27890928), and results in reduced catalytic efficiency (kcat/km) in an in vitro assay (PMID: 30684523), but has not been fully characterized and therefore, its effect on Abl1 protein function is unknown.

   
Technical Data 
Fusion Left Gene:                BCR(E14) 
Left Breakpoint:        hg19 chr22:23632600:+  
Right Gene:              ABL1(E2) 
Right Breakpoint:      hg19 chr9:133729451:+  
Mutation DNA Change:            c.944C>T
AA Change:               p.T315I
   
Product Information
Intended Use Research Use Only
Unit Size 1ug
Concentration Download for COA
Purity Download for COA
RNA electrophoresis Download for COA
Sanger sequencing

 


Figure 1. BCR-ABL1 (E14-E2) Fusion


Figure 2. ABL1 p.T315I

Storage -90~ -70℃
Expiry 12 months from the date of manufacture

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