免疫胶体金技术及其在临床诊断上的研究进展

综述了免疫胶体金技术的原理、特点以及斑点金免疫渗滤法、胶体金免疫层析法在临床诊断上的应用研究进展,并分析了该技术存在的问题及发展趋势。     

金属纳米颗粒对蛋白核小球藻生长活性的影响

研究了金属Fe、Ni纳米颗粒对蛋白核小球藻Chlorella pyrenoidosa生长活性的影响,探讨了金属纳米材料的生物安全性问题。结果表明：Fe、Ni金属纳米颗粒不仅能吸附在藻细胞表面,造成其团聚沉淀,而且还能进入细胞内部,引起细胞的形变和结构损伤,从而抑制了小球藻的正常生长,降低小球藻的生物量,对小球藻具有一定的毒性效应。     

小麦黄花叶病毒P2蛋白原核表达、抗血清制备及其在感病小麦细胞中的定位

通过RT PCR获得小麦黄花叶病毒(Wheat yellow mosaic virus, WYMV)扬州分离物P2基因,并进行序列分析。P2基因编码区含有2 635个核苷酸,编码一个由875个氨基酸组成的分子量72 kDa 的蛋白。在原核表达体系中,该基因的全长表达较困难,因此将P2基因的5′端和3′端各设计大约1 kb亚克隆到原核表达载体pMAL C2X中构建重组表达载体MBP P2N,MBP P2C,经IPTG诱导在大肠杆菌BL21(DE3)中表达MBP P2N和MBP P2C融合蛋白。MBP P2C融合蛋白经大量诱导、纯化、制备相应抗血清。用制备的抗血清可以有效检测WYMV病叶中的P2蛋白。免疫胶体金标记实验表明在感病WYMV的小麦叶片细胞膜状内含体结构中发现有大量胶体金颗粒特异性分布,表明P2蛋白可能与膜状内含体结构有关。     

检测南方水稻黑条矮缩病毒胶体金免疫试纸条的建立

由白背飞虱Sogatella furcifera(Horváth)传播的南方水稻黑条矮缩病毒(Southern rice blackstreaked dwarf virus,SRBSDV)是目前我国南方水稻上危害最严重的病毒,为开发简便、快速、准确的SRBSDV病毒检测技术和检测试剂,以感染SRBSDV的植物粗提液为免疫原,利用杂交瘤技术制备了2株抗SRBSDV的单抗(14A8和15G6),并利用制备的单抗建立了可快速、特异、灵敏地检测SRBSDV的胶体金免疫试纸条。结果表明,2株制备单抗的抗体类型及亚类均为Ig G1、kappa链,单抗腹水的间接ELISA效价均达到10~(-7);Western blot分析表明,2株单抗均与SRBSDV的外壳蛋白亚基有特异反应,而不与水稻黑条矮缩病毒(Rice black-streaked dwarf virus,RBSDV)反应。以制备14A8和15G6单抗分别为捕获抗体和胶体金标记抗体,开发成能在5 min内准确、特异地检测水稻植物和白背飞虱传毒介体体内SRBSDV的胶体金免疫试纸条;灵敏度分析表明,该检测试纸条的检测水稻病叶的灵敏度达到1∶6 400倍(g/m L),检测单头携毒白背飞虱的灵敏度达到1∶51 200倍(单头/μL)。田间样品检测结果表明,该试纸条的检测结果与RT-PCR的符合率达到100%。建立的SRBSDV胶体金免疫试纸条可对南方水稻黑条矮缩病毒进行快速、特异、灵敏的诊断和检测。     

纳米标记免疫层析法在农药残留检测中的应用研究进展

农药残留超标已成为影响农产品质量安全的重要问题,迫切需要探寻开发灵敏、准确、可靠、便捷且适用性强的农药残留快速检测方法。免疫层析法是将抗原抗体特异性免疫反应和色谱层析分离技术相结合的一种快速检测方法,其中,基于胶体金标记的免疫层析技术以其便捷、成本低、可视化等优点而受到普遍欢迎。近年来随着量子点、时间分辨荧光微球、上转换发光纳米粒子等新型纳米标记材料的出现,免疫层析技术得到了广泛发展。文章从标记类型（非共价作用标记及共价作用标记）及标记材料（胶体金、纳米碳、量子点、上转换发光纳米粒子、磁性纳米颗粒、时间分辨荧光微球及荧光乳胶颗粒）等方面,综述了不同纳米材料标记的免疫层析技术及其在农药残留检测领域的研究及应用进展,可为深入开展农药残留免疫层析技术研究提供参考。     

Reduction of soil heavy metal bioavailability by nanoparticles and cellulosic wastes improved the biomass of tree seedlings

The purpose of this study was to use zero‐valent iron nanoparticles (nZVI) and cellulosic wastes to reduce bioavailability of lead (Pb) and cadmium (Cd), and to establish Persian maple seedlings (Acer velutinum Bioss.) in contaminated soil. One‐year‐old seedlings were planted in pots filled with unpolluted soil. Lead [Pb(NO₃)₂] and Cd [Cd(NO₃)₂] were added with concentrations of 0 (Control), 100 (Pb100), 200 (Pb200), and 300 (Pb300) mg kg⁻¹ and 10 (Cd10), 20 (Cd20), and 30 (Cd30) mg kg⁻¹. Cellulosic wastes were mixed with soil at the same time of planting [four levels: 0, 10 (W1), 20 (W2), 30 (W3) g 100 g⁻¹ soil]. The nZVI was prepared by reducing Fe³⁺ to Fe⁰ and injected to pots [four levels: 0, 1 (N1), 2 (N2), and 3 (N3) mg kg⁻¹]. Height, diameter, biomass, tolerance index of seedlings, bioavailability of heavy metals in soil, and removal efficiency of amendments were measured. The highest values of seedling characteristics were observed in N3. The highest removal efficiency of Pb (Pb100: 81.95%, Pb200: 75.5%, Pb300: 69.9%) and Cd (Cd10: 92%, Cd20: 73.7%, Cd30: 68.5%) was also observed in N3. The use of nZVI and cellulosic waste could be a proper approach for seedling establishment in forests contaminated with heavy metals.     

以金磁微球为载体的H5N1 AIV免疫PCR检测方法的建立

【目的】将高特异性的抗原-抗体反应与高灵敏性的PCR扩增技术相结合,建立快速检测低浓度H5N1禽流感病毒(Avianinfluenzavirus,AIV)的免疫PCR方法。【方法】以pUC19为模板,采用5′端标记有生物素的引物进行PCR扩增,制备含有生物素的报告DNA分子。以金磁微球为固相吸附载体,通过亲和素-生物素的桥联作用,将含有生物素的报告DNA分子与生物素标记的抗AIVH5N1血凝素蛋白的检测抗体分子连接,H5N1AIV与检测抗体结合后,体外扩增报告DNA,间接放大低含量病毒信号,建立可有效检测微量H5N1AIV的免疫PCR方法。对建立的免疫PCR方法的最适报告DNA浓度、最适链亲和素工作浓度、灵敏度和特异性进行确定和评价。【结果】建立的免疫PCR方法最适报告DNA质量浓度为1ng/mL,最适链亲和素工作质量浓度为20ng/mL,该方法可成功检测到10-4EID50/mL的H5N1AIV,而且特异性良好。【结论】建立的以金磁微球为吸附载体的免疫PCR是一种灵敏度高、特异性好的检测微量H5N1AIV的方法。     

纳米SiO2表面改性及其对阿维菌素吸附性能的影响

采用硅烷偶联剂KH-570对纳米SiO2进行了表面接枝改性,并探讨了改性材料对阿维菌素的吸附性能。通过X射线衍射(XRD)、扫描电子显微镜(SEM)、傅立叶变换红外光谱(FTIR)等技术对表面改性纳米SiO2的结构和性能进行了分析。结果表明,纳米SiO2粒子经KH-570进行表面改性后,其分散性得以改善,对阿维菌素的包封率比改性前的大幅提高,提高率最高达92.6%。用KH-570改性的纳米SiO2可作为一种较为理想的新型生物农药载体。     

Yak interferon-alpha loaded solid lipid nanoparticles for controlled release

To explore the potential of a novel animal interferon formulation for controlled release, the yak interferon-alpha (IFN-α) glutathione S-transferase (GST) fusion protein was expressed in Escherichia coli (E. coli) and the purified recombinant IFN-α was encapsulated into solid lipid nanoparticles (SLN) by double emulsion solvent evaporation (w/o/w) method. The particle size and zeta potential of IFN-α-loaded SLN were 124.2 ± 10.2 nm and −11.2 ± 0.6 mV. The encapsulation efficiency of IFN-α and loading capacity of the SLN were 83.7 ± 4.5% and 1.73 ± 0.15%, respectively. In vitro release study and antiviral assay demonstrated that the IFN-α released from the SLN in a 16-day period exhibited antiviral activity in Madin-Darby bovine kidney (MDBK) cells against vesicular stomatitis virus (VSV), and showed a release pattern of an initial burst release followed by a sustained and slow release. Cytotoxicity assay in cell culture demonstrated that the SLN were not toxic. The results of this exploratory study suggest that the IFN-α-loaded SLN could be a useful formulation for controlled release in veterinary therapeutics.     

甲型流感病毒NP蛋白原核表达及其金标检测方法的建立

构建甲型流感病毒NP基因重组质粒,制备NP蛋白,建立甲型流感病毒胶体金检测方法。设计引物,扩增人工合成的甲型流感病毒株A(H5 N1)(GenBank登录号AY585439)NP DNA基因,构建pET-30 Xa/LIC-NP重组质粒,转化入原核表达系统E.coliBL21 Gold中进行表达和纯化。结果制备了纯度高达900 mL/L的甲型流感病毒NP融合蛋白,并初步建立了金标检测方法。