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Intein-mediated rapid purification and characterization of a novel recombinant agonist for VPAC2.

机译:内含子介导的VPAC2新型重组激动剂的快速纯化和表征。

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In order to obtain the recombinant VPAC2 agonist efficiently by intein-mediated single column purification, a gene encoding 32-amino acids peptide was designed, synthesized and cloned into Escherichia coli expression vector pKYB. The recombinant vector pKY-ROM was transferred into E. coli ER2566 cells and the target protein was over-expressed as a fusion to the N-terminus of a self-cleavable affinity tag. After the rMROM-intein-CBD fusion protein was purified by chitin-affinity chromatography, the self-cleavage activity of the intein was induced by beta-mercaptoethanol and the rMROM with the homogeneity over 95% was released from the chitin-bound intein tag. The recombinant linear rMROM competitively displaced [125I] PACAP38 on VPAC2 with a half-maximal inhibitory concentration (IC50) of 60 +/- 5 nM, whereas the IC50 of rMROM at human VPAC1 was observed up to 10 microM and no binding was detected at PAC1. rMROM stimulated the cAMP accumulation in Chinese hamster ovary (CHO) cells expressing the human VPAC2 with a half-maximal stimulatory concentration (EC50) of 0.6 nM, which was 500-fold less potent at VPAC1and had no activity on PAC1. An efficient production procedure of a novel recombinant VPAC2-selective agonist was established.
机译:为了通过内含蛋白介导的单柱纯化有效地获得重组VPAC2激动剂,设计,合成了编码32个氨基酸的肽的基因,并将其克隆到大肠杆菌表达载体pKYB中。将重组载体pKY-ROM转移到大肠杆菌ER2566细胞中,目标蛋白作为与可自我切割的亲和标签N端的融合体被过表达。通过甲壳素亲和层析纯化rMROM-intein-CBD融合蛋白后,β-巯基乙醇诱导了intein的自切割活性,并从几丁质结合的intein标签中释放了均一性超过95%的rMROM。重组线性rMROM在VPAC2上竞争性置换[125I] PACAP38,其半数抑制浓度(IC50)为60 +/- 5 nM,而在人VPAC1上rMROM的IC50高达10 microM,在PAC1。 rMROM刺激了表达人VPAC2的中国仓鼠卵巢(CHO)细胞中的cAMP蓄积,其最大刺激浓度(EC50)为0.6 nM,对VPAC1的作用强度降低了500倍,并且对PAC1没有活性。建立了新型重组VPAC2选择性激动剂的有效生产程序。

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