盐胁迫对珠美海棠和山定子膜保护酶系统的影响

实验以耐盐种珠美海棠(MaluszumiMats)和盐敏感种山定子[Malusbaccata(L.)Borkh]为试材,比较研究了在盐胁迫下叶片质膜透性、叶绿素和丙二醛(MDA)含量、膜保护酶超氧化物歧化酶(SOD)、过氧化氢酶(CAT)、过氧化物酶(POD)活性及根质膜透性的变化,为探索苹果属植物耐盐机制提供素材。结果表明,盐胁迫对根质膜透性没有明显的影响;但导致叶片质膜透性增加,盐敏感种山定子的质膜透性高于耐盐的珠美海棠。随盐胁迫加重,叶绿素a、b含量降低,叶绿素a/b比值增加,类胡萝卜素变化不明显。MDA含量随盐胁迫而升高,但珠美海棠低于山定子。山定子叶片中SOD、POD、CAT活性随盐胁迫加重而降低,而珠美海棠SOD活性在盐胁迫下保持稳定,POD、CAT活性增高。由此可见珠美海棠在盐胁迫条件下有活性较高的膜保护酶系统。     

禽流感病毒H5亚型主要保护性抗原在禽痘病毒中的高效表达

将H5亚型禽流感病毒血凝素HA基因克隆入插入载体pllS中获得重组转移质粒p11SH5A,通过酶切鉴定获得了预期的转移质粒p11SHSA,将质粒p11SHSA和野生禽痘病毒(wtFPV)共转染鸡胚成纤维细胞(CEF),通过蓝白斑筛选纯化得到重组病毒rFPV-11SH5A.以间接免疫荧光法证实,HA基因得到了表达.将该重组病毒rFPV-11SH5A以10(5)PFU/只免疫7日龄SPF鸡,于7、10、14、18、21d分别采血分离血清检测HI抗体,于免疫21d后用10(5)ELD50的野生病毒进行肌肉注射观察疫苗保护率.结果表明,该疫苗能提供100%的保护.     

细菌耐药颉颃剂的研究现状及应用

作者介绍了具有颉颃细菌耐药性作用的物质的研究应用进展情况，包括灭活酶抑制剂、药物渗透促进剂、外输泵抑制剂、细菌生物被膜抑制剂、抗菌药物增强剂、耐药质粒消除剂等。     

不同佐剂和免疫途径对柔嫩艾美耳球虫SO7抗原免疫保护效果的影响

利用PGEX-6P-1融合表达系统将SO7基因在大肠杆菌中进行融合表达,对表达产物进行初步纯化和复性,制备免疫原。分别使用不同剂量的人参总皂甙和重组γ-干扰素以及弗氏完全佐剂作为免疫佐剂,于5日龄、12日龄和19日龄对雏鸡进行3次免疫,同时设立蛋白口服免疫组、蛋白皮下注射免疫组、卵囊口服免疫组、未免疫未攻毒组和未免疫攻毒组作对照,于26日龄用105个柔嫩艾美耳球虫卵囊进行攻毒,8d后扑杀,对各组的存活率、相对增重率、病变减少率、相对卵囊产量和抗球虫指数ACI等指标进行统计分析,比较免疫保护效果。与非免疫攻毒组以及不加佐剂的免疫攻毒组相比,佐剂使用后各组的增重、病变记分、相对卵囊产量、ACI等指标均有一定的改善,对柔嫩艾美耳球虫的人工感染可以提供部分保护。3种佐剂中,γ-干扰素和人参总皂甙能增强重组蛋白的免疫保护效果,且佐剂的剂量对免疫保护的效果有一定的影响,以5000Uγ-干扰素效果最佳,效果与E.tenella活卵囊免疫相当,弗氏完全佐剂的免疫增强效果不明显。单独使用重组蛋白皮下注射或口服免疫,虽有一定的保护作用,但不明显。一定剂量的γ-干扰素对SO7抗原的免疫保护效果起明显的增强作用,是一个具有很好临床应用前景的新型佐剂。     

钠离子对仔猪小肠刷状缘膜囊二肽跨膜转运的影响

为研究Na 在仔猪小肠Gly-Pro跨膜转运中的作用,采用同位素示踪及体外孵育技术,观察在不同Na 浓度梯度条件下Gly-Pro在仔猪小肠刷状缘膜囊(brush border membrane vesicles,BBMV)的跨膜转运量。结果表明:(1)用K 替代Na ,并没有降低Gly-Pro在BBMV中的转运量,在孵育前20min时间内,Gly-Pro的转运量稍稍提高;(2)Na 可使BBMV对L-丙氨酸的转运量提高到4.6倍,但不影响Gly-Pro的转运;二氢骆驼蓬碱显著地降低L-丙氨酸的转运,但对Gly-Pro的转运无影响。研究提示,Gly-Pro在仔猪小肠BBMV体系中的转运与Na 不存在依赖性的关系。     

增强猪传染性胸膜肺炎灭活苗对小鼠保护力的研究

为了提高猪传染性胸膜肺炎灭活苗的保护力,本研究利用基因重组技术表达了猪传染性胸膜肺炎放线杆菌6种主要致病因子蛋白:rApxⅠ、rApxⅡ、rApxⅢ、rApxⅣ、rApfa和rOMP。设立试验Ⅰ组(灭活苗),试验Ⅱ组(灭活苗、rApxⅠ、rApxⅡ、rApxⅢ和rOMP),试验Ⅲ组(灭活苗、rApxⅠ、rApxⅡ、rApxⅢ和rApxⅣ),试验Ⅳ组(灭活苗、rApxⅠ、rApxⅡ、rApxⅢ和rApfa)和空白对照组(PBS),每组26只BALB/c小鼠,分3次免疫,每次间隔2周,每周检测血清抗体水平,在免疫后第2周、第4周和第5周,MTT法检测脾脏T细胞增殖水平及ELISA法测定IFN-γ分泌水平。在第3次免疫后的第7 d,将每组剩余20只小鼠平均分成2组,分别以APP1型菌(5×10~9 CFU)和APP7型菌(1×10~(11) CFU)进行攻毒保护试验。结果表明,向灭活苗中添加重组亚单位成份可以提高机体的细胞免疫和体液免疫水平,并能提高灭活苗的交叉保护率;试验Ⅱ组的ApxⅠ和OMP抗体水平以及细胞免疫水平均显著高于其它各组(p<0.05),对于APP1和APP7型菌的攻毒也提供了明显优于其它各组的保护结果,试验Ⅲ、Ⅳ组的细胞、体液免疫水平及保护率较试验Ⅰ组也有所提高。结果显示出ApxⅠ、OMP抗体水平和细胞免疫水平与攻毒保护率之间存在着正相关性,向灭活苗中加入重组蛋白成份可以提高疫苗的交叉保护,试验Ⅱ组通过激活体液免疫和细胞免疫,对两个血清型APP的攻击提供了很好的保护作用,从而为猪传染性胸膜肺炎新型疫苗的研制提供参考。     

Changes in antioxidative system and membrane damage of lettuce in response to salinity and boron toxicity

Individual and combined effects of salinity and B toxicity on growth, the major antioxidant enzymes (superoxide dismutase, SOD; catalase, CAT; ascorbate peroxidase, APX) activities, ascorbic acid, proline, and H₂O₂ accumulation, and stomatal resistance (SR), malondialdehyde (MDA), membrane permeability (MP) and the concentrations of sodium (Na), chloride (Cl) and boron (B) of lettuce were investigated. Boron toxicity and salinity reduced growth of lettuce plants. Under B toxicity, B concentration of the plants was increased, but in the presence of NaCl, the concentration of B was significantly reduced. Sodium and Cl concentrations were increased in B + NaCl and NaCl treatments. Membrane damage was more pronounced in NaCl and B + NaCl treatments. Stomatal resistance of the plants was significantly increased by salinity treatments. The accumulation of proline and ascorbic acid was the highest in the B + NaCl treatment. In general, stress conditions significantly increased H₂O₂ and antioxidant enzyme (SOD, CAT and APX) activities. The present results indicate that stomatal closure is an important response of lettuce against NaCl and B + NaCl stress. Furthermore NaCl and B + NaCl toxicity-induced oxidative stress in lettuce resulting in lipid peroxidation and membrane damage. Increased antioxidant enzyme activities and also accumulation of ascorbic acid and proline are involved in order to overcome B- and NaCl-induced oxidative stress.     

The latent gene expression of Epstein-Barr virus in nasopharyngeal carcinoma

AIM: To examine the latent membrane protein 1(LMP1)-DNA sequence in nasopharyngeal carcinoma(NPC) and detect mRNA expression of LMP1,EBNA1,EBNA2,and to explore the relationship between EBV infectious status,expression products and NPC carcinogenesis.METHODS: LMP1 DNA was detected in NPC by PCR.Direct sequence was applied to analyze the difference between NPC-LMP1-DNA and B95-8- LMP1-DNA.mRNA expressions of LMP1,EBNA1,EBNA2 in NPC were detected by nested RT-PCR.RESULTS: LMP1 DNA existed in all 47 NPC tissues.Several single nucleotide variations were found between NPC-LMP1-DNA and B95-8- LMP1-DNA.The notable variation was the lost of XhoⅠrestriction site in NPC.Direct sequence showed 30 bp deletion in NPC.The mRNA expressions of LMP1,EBNA1 and EBNA2 in NPC were 76.6%,80.0% and 74.5% respectively by nested RT-PCR.The expression of EBNA1 in NPC was promoted by Q promoter while the expression of EBNA1 in B95-8 was promoted by C promoter.CONCLUSION: The way of EBV involved in NPC is complex.Latent genes such as LMP1,EBNA1 and EBNA2 as well as early lytic gene BARF1 may all play certain roles in NPC carcinogenesis.     

Antiproliferation effects of 188Re labeled monoclonal antibody on prostate cancer cells in vitro

AIM: To investigate the effect of 188Re labeled monoclonal antibody on prostatic specific membrane antigen 7E11C5.3,radioimmunotherapy for the treatment of human prostate cancer cell line LNCaP in vitro.METHODS: 188Re-7E11C5.3 was prepared by direct 2-mercaptoethanol reduction method.Labeling efficiency and radiochemical purity was measured by paper chromatography.Immunoreactive fraction was determined by linear extrapolation.Cytotoxicity to LNCaP cells was determined by MTT assay.RESULTS: The labeling yield of 188Re-7E11C5.3 was (93.16±2.18)%,the radiochemical purity was (95.62±0.48)%,and the immunoreactive fraction was (74.86±1.86)%.The inhibitory effect of 188Re-7E11C5.3 on cell proliferation of LNCaP cells was significantly higher than that of 188Re-mIgG or 188ReO-4.The 50% inhibitory doses (IC50) of 188Re-7E11C5.3,188Re-mIgG,and 188ReO-4 were (23.38±3.73)×107 Bq/L,(59.21±8.02)×107 Bq/L and (68.89±10.91)×107 Bq/L,respectively.CONCLUSION: 188Re-7E11C5.3 can effectively inhibit the growth of in vitro cultured prostate cancer cells and shows much potential for prostate cancer radioimmunotherapy.     

水分胁迫对抗旱性不同小麦品种叶片光合及根呼吸等生理特性的影响

以两个抗旱性不同的小麦品种西农1043、陕253为材料，采用盆栽与水培试验相结合的方式，研究水分亏缺对小麦不同生育期叶片光合及根呼吸速率等生理指标的影响。结果表明：相同水分处理下，抗旱品种西农1043与水分敏感品种陕253相比，具有较高的光合和根呼吸速率、以及相对较高的保护酶活性；水分胁迫下，两个小麦品种叶片光合和根呼吸速率及苗期叶保护酶活性均降低；两种水分处理下抗旱性强的西农1043根呼吸所占光合的比例相对高于陕253。