We cloned the dok1 and dok5 full-length cDNA and expressed their PTB domains, and then the recombinant proteins were purified by affinity, anion exchange and gel filtration chromatography.

 
  • 我们克隆表达了dok1和dok5蛋白,并表达纯化了dok1和dok5的PTB结构域。 经Biacore实验发现,dok1 PTB结构域可特异识别来自Ret的磷酸肽,但不与Shc和Irs1 PTB识别的TrkA和IL-4R磷酸肽结合;
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