摘要
目的:研究具有生物学活性的人防御素2(HBD 2)多肽在大肠杆菌中的原核高效表达的可行性及融合表达蛋白的分离纯化技术。方法:PCR扩增不含前导序列的HBD 2成熟肽的编码框全长的cDNA片段(smHBD 2-cDNA),利用B g lⅡ和B amHⅠ同尾酶构建多拷贝串联的nsmHBD 2-cDNA的克隆载体,利用N colⅠ和H indⅢ限制性内切酶构建融合表达载体pET 32-nsmHBD 2-cDNA,在大肠杆菌中BL 21(DE 3)中诱导表达含HBD 2的融合蛋白,SDS-PAGE分析产量。可溶蛋白经亲和层析、肠激酶酶切、离子交换层析等方法分离、纯化HBD 2多肽。采用液体培养法,测定重组人β防御素2对大肠杆菌的抑菌活性。结果:构建了n为1、2、4或8倍的多拷贝串联nsmHBD 2-cDNA表达载体,1、2和4倍smHBD 2-cDNA的可溶蛋白比例分别为52%、48%和31%;而8倍HBD 2-cDNA几乎不含可溶蛋白,目标蛋白以包含体形式表达,集中在不可溶部分。重组HBD 2对E.coli K 12 D 31有较强的抑制作用,在终浓度约为0.4至0.5μg/m l时,90%细胞的生长被抑制。结论:采用融合表达、多拷贝串联表达方式,可增加产物长度以弱化蛋白酶的降解作用,也减弱了目标蛋白产物对宿主的毒性;适当的多拷贝串联基因可以提高HBD 2的产量,但拷贝数过高会影响重组蛋白表达产量,且易形成不溶蛋白;在大肠杆菌中可达到具有生物学活性的HBD 2多肽的原核高效表达。
Objective: To demonstrate the possibility of high-level expression of bioactive human beta-defensin-2 (hBD2) in E.coli, and to purify the recombinant hBD2. Methods: DNA fragment containing mature hBD2 coding region (smhBD2-cDNA) was amplified by PCR, multiple copies of smhBD2-cDNA were linked using Bgl Ⅱ and BamH Ⅰ enzymes, pET32-nsmHBD2-cDNA with 1, 2, 4, or 8 copies of smhBD2-cDNA was constructed. The soluble and insoluble hBD2 proteins were separated and analyzed by SDS-PAGE analysis. The soluble protein underwent a separation process containing affinity chromatography, enterokinase digestion and ion exchange chromatography to get the recombinant hBD2 peptide. The bioactivity of recombinant hBD2 was examined by bacteria-inhibition tests in liquid culture. Results: The plasmids pET32-nsmHBD2-cDNA with 1, 2, 4 copies of smhBD2-cDNA were constructed and the expressed soluble protein accounted for 52%, 48%, and 31% respectively. The plasmids with 8 copies expressed mainly insoluble protein with few in soluble form. The growth of E.coli K12D31 was dramatically suppressed with a inhibition rate of 90%, when the final concentration of recombinant hBD2 reached between 0.4 to 0.5 μg/ml. Conclusion: Fusion expression of human β-defensin-2 with multiple joined genes in E.coli could increase the expression of hBD2.
出处
《浙江大学学报(医学版)》
CAS
CSCD
2006年第6期585-589,共5页
Journal of Zhejiang University(Medical Sciences)
基金
国家自然科学基金资助项目(30070854)
浙江省科技厅基金项目(001103241)
关键词
防御素类/遗传学
大肠杆菌/遗传学
基因表达
Β-防御素
抗菌肽
原核表达
亲和层析
融合蛋白
Defensins/genetics
Escherichia coli/genetics
Gene expression
Human β-defensin 2
Antimicrobial peptide
Prokaryotic expression
Affinity chromatography
Fusion protein
