Gullo Charles A, Ge Feng, Cow Geraline, Teoh Gerrard
Department of Clinical Research (DCR), Cancer Immunology Laboratory, Singapore General Hospital (SGH), Outram Road, Singapore 169608, Singapore.
Cancer Cell Int. 2008 Apr 29;8:4. doi: 10.1186/1475-2867-8-4.
Truncated variants of Ku86 protein have previously been detected in 86% to 100% of freshly isolated patient multiple myeloma (MM) cells. Since, the Ku70/Ku86 heterodimer functions as the regulatory subunit of the DNA repair enzyme, DNA-dependent protein kinase, we have been interested in the altered expression and function of Ku86 variant (Ku86v) proteins in genome maintenance of MM.
Although, a number of studies have suggested that truncated forms of Ku proteins could be artificially generated by proteolytic degradation in vitro in human lymphocytes, we now show using whole cell immunoblotting that the RPMI-8226 and SGH-MM5 human MM cell lines consistently express full-length Ku86 as well as a 69-kDa Ku86v; a C-terminus truncated 69-kDa variant Ku86 protein. In contrast, Ku86v proteins were not detected in the freshly isolated lymphocytes as was previously reported. Data also indicates that the Ku86v was not generated as a result of carbohydrate modification but that serine proteases may act on the full-length form of the protein.
These data confirm that MM cells contain bona fide Ku86v proteins that were generated intracellularly by a post-transcriptional mechanism, which required proteolytic processing.
先前在86%至100%的新鲜分离的患者多发性骨髓瘤(MM)细胞中检测到Ku86蛋白的截短变体。由于Ku70/Ku86异二聚体作为DNA修复酶(DNA依赖性蛋白激酶)的调节亚基,我们一直对Ku86变体(Ku86v)蛋白在MM基因组维持中的表达和功能改变感兴趣。
尽管许多研究表明,Ku蛋白的截短形式可能是在体外人淋巴细胞中通过蛋白水解降解人工产生的,但我们现在使用全细胞免疫印迹法表明,RPMI-8226和SGH-MM5人MM细胞系持续表达全长Ku86以及一种69 kDa的Ku86v;一种C末端截短的69 kDa变体Ku86蛋白。相比之下,如先前报道,在新鲜分离的淋巴细胞中未检测到Ku86v蛋白。数据还表明,Ku86v不是碳水化合物修饰的结果,而是丝氨酸蛋白酶可能作用于该蛋白的全长形式。
这些数据证实,MM细胞含有真正的Ku86v蛋白,其通过转录后机制在细胞内产生,这需要蛋白水解加工。
Zotero 插件
