抗人角蛋白全IgG基因真核表达载体的构建及表达

目的：构建抗角蛋白抗体基因的真核表达载体，并在CHO(dhfr^-)细胞中表达。方法：从含抗角蛋白抗体基因的原核Fab表达载体中，扩增VH及VL基因。以回收的PCR产物为模板，用重叠PCR扩增带有前导序列的VH、VL基因。经XbaⅠ/BamHⅠ和XhoⅠ/HindⅢ酶切后，分别插入真核表达载体pWD中，构建重组载体pWDkH。经PCR和测序鉴定正确后，用lipofectAMINE2000转染CHO(dhfr^-)细胞。取培养上清检测抗人角蛋白全IgG的表达。结果：构建了抗人角蛋白基因的真核表达载体pWDkH，并在CHO(dhfr^-)细胞中表达：结论：在CHO(dhfr^-)细胞中成功地表达了具有抗原结合活性的抗人角蛋白IgG，为其临床应用奠定了基础。

Construction and expression of eukaryotic expression vector for intact IgG against human keratin

AIM: To construct an eukaryotic expression vector containing the gene of anti-keratin antibody and express it in CHO(dhfr(-)) cells. METHODS: Both the V(L) and V(H) genes of an anti-keratin Fab from a phage display library were amplified by PCR.Using PCR product as the template, the V(kappa) and V(H) genes with the leader sequences (named L(kappa) and L(H) respectively) were amplified by overlapping PCR.After digested with endonuclease Xba I/BamH I and Xho I/Hind III, L(kappa) and L(H) genes were inserted into pWD digested with Xba I/BamH I and Xho I/Hind III, respectively to construct pWDkappaH.After PCR and sequencing, the expression plasmid pWDkappaH was transfected into CHO (dhfr(-)) cells. The culture supernatant of the transfected cells was collected and assayed for IgG activity. RESULTS: The eukaryotic expression vector pWDkappaH was constructed successfully and expressed in CHO(dhfr(-)) cells. The expression of intact IgG against keratin was identified by ELISA and RT-PCR. CONCLUSION: The successful expression of intact IgG against keratin lays the foundation for its clinical application.