Gene cloning, expression and polyclonal antibody preparation of Rab3A for protein interaction analysis

被引:6
|
作者
Tang, Xia [1 ]
Chen, Jia [1 ]
Wang, Ying [1 ]
Wang, Xianchun [1 ]
机构
[1] Hunan Normal Univ, Coll Life Sci, Key Lab Prot Chem & Dev Biol, Minist Educ, Changsha 410081, Hunan, Peoples R China
来源
SPRINGERPLUS | 2016年 / 5卷
基金
中国国家自然科学基金;
关键词
Rab3A; Fusion expression; Polyclonal antibody; Gel protein recovery; Protein interaction; ESCHERICHIA-COLI; NEUROTRANSMITTER RELEASE; BINDING PROTEIN; TARGET PROTEIN; SYNAPTOTAGMIN; PURIFICATION; EFFECTOR; EXOCYTOSIS; SUBFAMILY; MEMBRANES;
D O I
10.1186/s40064-016-3330-y
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
Background: Rab3A is a GTP-binding protein and plays critical roles in the regulation of synaptic vesicle exocytosis. Up to date, how Rab3A participates in such a regulatory process is not completely clear. Results: In this report the Rab3A gene from Rattus norvegicus was cloned and heterologously expressed in E. coli using pCold-TF expression vector with folding capacity. Due to the presence of His-tag sequence on the N-terminal side, Rab3A fusion protein was purified to greater than 95 % purity with a single Ni-affinity purification step. After the Rab3A fusion protein was used to immunize mice, an anti-serum against Rab3A with a titer of about 6000 was generated. Western blot analysis indicated that the prepared polyclonal antibody could recognize both Rab3A fusion protein and native Rab3A protein. To remove the tag sequence, thrombin was used to cleave the Rab3A fusion protein, followed by SDS-PAGE to separate the cleavage products. Using the gel protein recovery strategy with a Micro Protein PAGE Recovery Kit, the de-tagged Rab3A protein of electrophoretic purity was prepared. Conclusions: The present work not only prepared the ground for the study on Rab3A-mediated protein interactions, but also provided systematic experimental methods referable for the similar studies.
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页数:7
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