【摘要】 目的: 获取重组鼠IL?28(mIL?28)纯化蛋白,制备多克隆抗体。方法: 用PCR技术扩增鼠IL?28成熟蛋白的编码序列,克隆入原核表达载体pET?30,构建融合表达载体pET?30a?mIL?28,转化大肠埃希菌 BL21(DE3),以IPTG诱导表达IL?28融合蛋白,经镍柱亲和层析纯化,然后免疫6~8周龄鸡,制备多克隆抗体,采用ELISA 检测抗体效价。结果: 成功构建了表达载体pET?30a?mIL?28,DNA序列测定结果与预期结果一致。在37℃培养条件下,IPTG诱导表达的IL?28融合蛋白进行 SDS?PAGE电泳分析,发现其与融合蛋白的理论计算值一致,免疫鸡后收获抗血清, ELISA 显示抗体效价具有高度特异性。结论: 获得了重组鼠IL?28纯化蛋白,制备了鼠IL?28多克隆抗体,为进一步深入研究IL?28的生物活性及其应用打下基础。
高级职称论文发表 中国论文网BlG(v,]&@x;y@N+G8\&wl0【关键词】 白细胞介素?28; 大肠埃希菌; 蛋白质纯化; 抗体制备
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p0 [Abstract]Objective: To obtain purified recombinant interleukin?28 of mouse(mIL?28) and prepare its polyclonal antibody. Methods: The cDNA fragment coding for mature mIL?28 protein was amplified by PCR and cloned into vector pET?30 to construct fusion expression vector pET?30a?mIL?28.After pET?30a?mIL?28 was transformed into E.coli BL21(DE3), the bacteria were induced by IPTG.The expressed mIL?28 fusion protein was purified by Ni?NTA affinity chromatography.Six to eight weeks old chickens were immunized with the purified protein for obtaining the antiserum.The titers of antibodies were measured by ELISA. Results: The DNA sequencing showed that the expression vector pET?30a?mIL?28 was constructed successfully.After induced by IPTG,the expressed mIL?28 fusion protein in E.coli cultured at 37℃ appeared a single band on SDS?PAGE.The result of ELISA indicated that the prepared polyclonal antibody had high titer and specificity. Conclusion: The purified recombinant interleukin?28 of mouse and polyclonal antibody have been acquired.
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W%N9H0qj9t2EA7m{0 [Key words] interleukin?28;Escherichia coli;protein purification; antibody preparation
y X'lbN:a B:] U0bH7x}vc0 2003年, Sheppard 等[1 ] 和Kotenko 等[2]先后报道了一组新型的白细胞介素IL?28A,IL?28B,IL?29(又称为IFN?λ2,IFN?λ3,IFN?λ1),其中IL?28A 和IL?28B合称IL?28。IL?28在结构和(或)功能上与IL?10家族和I型干扰素(IFN)家族相似,因与IFN家族更接近,所以有学者将其命名为Ⅲ型干扰素。小鼠的 IFN?λ 家族仅发现 2个成员,即IL?28A和IL?28B [3]。
中国论文网;~!@L(p vP.B中国论文网r\+T AL4X 本实验在克隆全长鼠IL?28 cDNA 的基础上,构建了重组鼠IL?28的原核表达载体,在大肠埃希菌中进行表达、纯化,为进一步深入研究IL?28的生物活性及其应用打下基础。
高级职称论文发表 )V5M!vL0`pR.`'P,i0中国论文网*asW!SpRW5@ 1 材料和方法
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