靶向DC-SIGN的Le(x)-OVA抗原的制备

目的制备用于靶向DC-SIGN受体的Le(x)寡糖介导的靶向抗原。方法利用Su lfo-SMCC异源双功能交联试剂交联链霉亲和素(streptavid in,SA)和模式抗原卵白蛋白(ovalbum in,OVA),再利用SA与生物素高亲和力结合的特性,将SA-OVA复合物与生物素修饰的Le(x)寡糖反应,由此获得由Le(x)寡糖介导的靶向抗原Le(x)-OVA复合物。结果应用SDS-PAGE蛋白质电泳和W estern免疫印迹方法证实SA与OVA蛋白成功交联,ELISA方法证实SA-OVA复合物中的SA仍具有与生物素反应的功能,根据SA-OVA复合物与生物素修饰的Le(x)寡糖饱和反应的比例,获得所需要的靶向抗原Le(x)-OVA复合物。结论获得Le(x)寡糖介导的靶向抗原Le(x)-OVA复合物,为进一步研究经由DC-SIGN靶向后的抗原特异性免疫应答奠定了基础。

西妥昔单抗-β葡萄糖苷酶偶联物的制备及鉴定

目的制备西妥昔单抗-β葡萄糖苷酶偶联物并鉴定其酶活性与抗体活性。方法采用4-(N-马来酰亚胺甲基)环己烷-1-羧酸磺酸基琥珀酰亚胺酯钠盐(Sulfo-SMCC)将西妥昔单抗、β-葡萄糖苷酶进行共价交联。采用非还原型聚丙烯酰胺凝胶电泳(SDS-PAGE)、比色法、间接免疫荧光法对偶联物进行鉴定并检测β-葡萄糖苷酶、西妥昔单抗的活性。结果在电泳图上可分别见到β葡萄糖苷酶、西妥昔单抗、西妥昔单抗-β葡萄糖苷酶偶联物的清晰条带。比色法测定结果显示,西妥昔单抗-β-葡萄糖苷酶偶联物的酶活性低于β-葡萄糖苷酶(U/L:672.97±46.19 vs869.50±57.28,t=5.972,P<0.05),但仍保持良好的酶活性。在荧光显微镜下可见到与偶联物共同作用的人膀胱癌EJ细胞带有红色荧光。结论 Sulfo-SMCC可成功将西妥昔单抗、β-葡萄糖苷酶偶联,且偶联物仍能保持良好的酶活性与抗体活性。

人工诱骗子的入核分布对核因子-κB活性的调控作用

探讨了由核定位信号(NLS)多肽介导的核因子-κB(NF-κB)寡核苷酸诱骗子(ODNs decoy)进入HeLa细胞核的效率,以及对细胞核内NF-κB活性的调控作用。利用双功能交联剂(Sulfo-SMCC)共价交联末端氨基修饰的ODNs decoy和末端巯基修饰的NLS多肽,形成NLS多肽共价连接的ODNs decoy。依靠TransME转染试剂的辅助转染NLS-ODNs decoy进入HeLa细胞,用荧光显微镜观察荧光标记的NLS-ODNs在细胞内的分布。用MTT法检测HeLa细胞的活力,以凝胶迁移实验(EMSA)检测TNF-α诱导的HeLa细胞核抽提物中NF-κB的活性。结果表明,NLS多肽成功地连接到ODNs decoy上,NLS-ODNs可高效入核,入核率达到17.9%。转染NLS-ODNs进入HeLa细胞,对细胞活力无明显影响,而显著抑制核内NF-κB的活性。结果表明NLS多肽可提高ODNs decoy的入核效率,显著增强诱骗子对NF-κB活性的抑制效果。

Cross-linked self-assembling peptide scaffolds

Self-assembling peptides （SAPs） are synthetic bioinspired biomaterials that can be feasibly multi-functionalized for cell transplantation and/or drug delivery therapies. Despite their superior biocompatibility and ease of scaling-up for production, they are unfortunately hampered by weak mechanical properties due to transient non-covalent interactions among and within the self-assembled peptide chains, thus limiting their potential applications as fillers, hemostat solutions, and fragile scaffolds for soft tissues. Here, we have developed and characterized a cross-linking strategy that increases both the stiffness and the tailorability of SAP hydrogels, enabling the preparation of transparent flexible threads, discs, channels, and hemispherical constructs. Empirical and computational results, in close agreement with each other, confirmed that the cross-linking reaction does not affect the previously self-assembled secondary structures. In vitro tests also provided a first hint of satisfactory biocompatibility by favoring viability and differentiation of human neural stem cells. This work could bring self-assembling peptide technology to many applications that have been precluded so far, especially in regenerative medicine.