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作 者:张俊彦[1] 谢捷[1] 周远[1] 钟文涛[1] 龚兴国[1]
出 处:《中国药学杂志》2005年第12期943-946,共4页Chinese Pharmaceutical Journal
基 金:国家科技创新基金项目(03C26213300586)
摘 要:目的表达高纯度具有激酶活性的Src蛋白,为抗肿瘤药物研究提供蛋白质靶标。方法利用高效表达质粒pGEX-KT克隆v-src全基因,诱导表达得到的GST-Src融合蛋白经GlutationeSepharose4B亲和层析柱纯化后,采用Westernblotting和以polyGlu:Try(4:1)为底物的ELISA法鉴定其免疫原性和酪氨酸激酶活性。结果GST-Src蛋白表达量约占菌体总蛋白的30%,其中包涵体与可溶性蛋白的表达量分别约13.5和2mg·L-1,纯度分别约98%和85%,比活约1.13和0.62nmol·min-1·mg-1。结论本法表达的GST-Src融合蛋白表达量高、纯化效果好,且具有较高的激酶比活。OBJECTIVE: To clone and express the active v-Src protein, provide a PTK source for screening anti-tumor agents via Src inhibitors. METHODS: The pGEX-KT vector was employed in the cloning of v-src gene. The expressed protein was purified, using GSH Sepharose 4B, and its characteristics were identified by Western blot analysis and ELISA technique. RESULTS: The amount of GST-Src protein expressed from BL21 (DE3)pLysS culture exceeded 30% in relation to the coproteins. In 1 L medium culture, approximately 2 mg GST-Src fusion proteins with 85% purity and 13.5 mg GST-Src inclusion bodies with 98% purity were obtained. More-over, their tyrosine kinase activies reached about 0.62 nmol·min-1·mg-1 and 1.13 nmol·min-1·mg-1, respectively. CONCLUSION: The GST-Src fusion protein expressed in this study was of high product, easy to be purified and prefer-able in the kinase activity.
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