Kayes S G, Shaneyfelt R C, Monteiro C, O'Brien J J
Department of Structural and Cellular Biology, College of Medicine, University of South Alabama, Mobile 36688-0002, USA.
J Parasitol. 1998 Aug;84(4):764-70.
To evaluate the immune responses of mice vaccinated intramuscularly with naked DNA encoding a single parasite-derived gene, sufficient quantities of protein are necessary for use in the immunological assays. A plasmid carrying the cDNA encoding the entire sequence for the 28-kDa Schistosoma mansoni glutathione S-transferase (Sm28GST) was used as a source of naked DNA to vaccinate mice. Using polymerase chain reaction employing custom primers to add Eco RI and Hind III restriction sites at the 5' and 3' ends, respectively, a 651-bp fragment was amplified from the vaccine plasmid. This product was isolated, ligated into the pFastBac HTb donor plasmid containing a 6X histidine (6X-his) tag, and transposed into the baculovirus expression vector system. Following blue white selection screening, high molecular weight DNA was isolated and transfected in Sf21 insect ovary cells using a liposomal preparation. Culture medium containing infective virus particles was used to infect a series of Sf21 cultures and the cells were lysed after 3-5 days. The lysates were subjected to immobilized metal (Ni-NTA) affinity chromatography from which the 6X-his-tagged recombinant Sm28GST was eluted in 250 mM imidazole. The eluted protein was probed with a polyclonal rabbit antibody specific for the Sm28GST and subsequently recognized using a monoclonal antibody specific for the 6X-his tag following concentration of the pooled fractions. Mice were vaccinated intramuscularly with purified plasmid DNA encoding either the Sm28GST or firefly luciferase. Skin tests performed using recombinant Sm28GST were positive in only those mice vaccinated with naked DNA encoding the Sm28GST gene. In a different group of experimental mice, only sera from mice vaccinated with naked DNA encoding Sm28GST contained IgG-specific anti-Sm28GST antibodies at 14 days postvaccination, and at 42 days the levels were suggestive of an anamnestic response. These results suggest that naked DNA vaccination of mice is capable of inducing both antigen-specific cell-mediated and humoral immune responses against Sm28GST and further strengthen the case for this antigen being a vaccine candidate.
为了评估经肌肉注射编码单个寄生虫衍生基因的裸DNA疫苗接种的小鼠的免疫反应,在免疫分析中需要足够量的蛋白质。携带编码曼氏血吸虫28 kDa谷胱甘肽S-转移酶(Sm28GST)完整序列的cDNA的质粒用作裸DNA来源来给小鼠接种疫苗。使用聚合酶链反应,采用定制引物分别在5'和3'端添加Eco RI和Hind III限制性位点,从疫苗质粒中扩增出一个651 bp的片段。该产物被分离出来,连接到含有6X组氨酸(6X-his)标签的pFastBac HTb供体质粒中,并转座到杆状病毒表达载体系统中。经过蓝白斑筛选,分离出高分子量DNA,并使用脂质体制剂转染Sf21昆虫卵巢细胞。含有感染性病毒颗粒的培养基用于感染一系列Sf21培养物,3-5天后细胞被裂解。裂解物进行固定化金属(Ni-NTA)亲和层析,6X-his标签的重组Sm28GST在250 mM咪唑中被洗脱。洗脱的蛋白质用针对Sm28GST的多克隆兔抗体进行检测,随后在合并的级分浓缩后使用针对6X-his标签的单克隆抗体进行识别。小鼠经肌肉注射纯化的编码Sm28GST或萤火虫荧光素酶的质粒DNA进行接种。使用重组Sm28GST进行的皮肤试验仅在接种编码Sm28GST基因的裸DNA的小鼠中呈阳性。在另一组实验小鼠中,仅接种编码Sm28GST的裸DNA的小鼠血清在接种后14天含有IgG特异性抗Sm28GST抗体,在42天时这些水平提示有回忆反应。这些结果表明,小鼠的裸DNA疫苗接种能够诱导针对Sm28GST的抗原特异性细胞介导和体液免疫反应,并进一步支持该抗原作为疫苗候选物的理由。
