Expression of Anti-Lipopolysaccharide Factor Isoform 3 in Chlamydomonas reinhardtii Showing High Antimicrobial Activity     

Anguo Li  Ruihao Huang  Chaogang Wang  Qunju Hu  Hui Li  Xiao Li 《Marine drugs》2021,19(5)

Antimicrobial peptides are a class of proteins with antibacterial functions. In this study, the anti-lipopolysaccharide factor isoform 3 gene (ALFPm3), encoding an antimicrobial peptide from Penaeus monodon with a super activity was expressed in Chlamydomonas reinhardtii, which would develop a microalga strain that can be used for the antimicrobial peptide production. To construct the expression cluster, namely pH2A-Pm3, the codon optimized ALFPm3 gene was fused with the ble reporter by 2A peptide and inserted into pH124 vector. The glass-bead method was performed to transform pH2A-Pm3 into C. reinhardtii CC-849. In addition to 8 μg/mL zeocin resistance selection, the C. reinhardtii transformants were further confirmed by genomic PCR and RT-PCR. Western blot analysis showed that the C. reinhardtii-derived ALFPm3 (cALFPm3) was successfully expressed in C. reinhardtii transformants and accounted for 0.35% of the total soluble protein (TSP). Furthermore, the results of antibacterial assay revealed that the cALFPm3 could significantly inhibit the growth of a variety of bacteria, including both Gram-negative bacteria and Gram-positive bacteria at a concentration of 0.77 μM. Especially, the inhibition could last longer than 24 h, which performed better than ampicillin. Hence, this study successfully developed a transgenic C. reinhardtii strain, which can produce the active ALFPm3 driven from P. monodon, providing a potential strategy to use C. reinhardtii as the cell factory to produce antimicrobial peptides.  相似文献   

The role of ear environment in postharvest susceptibility of maize to toxigenic Aspergillus flavus     

Samuel K. Mutiga  Nelson Chepkwony  Owens A. Hoekenga  Sherry A. Flint‐Garcia  Rebecca J. Nelson 《Plant Breeding》2019,138(1):38-50

A kernel screening assay (KSA) was used to assess the genetic and environmental effects on the vulnerability of maize to aflatoxin accumulation. Kernels of 26 inbred lines that had been grown in seven environments, and 190 lines of the Intermated B73xMo17 (IBM) population grown in one location in the United States, were inoculated with a toxigenic strain of A. flavus and incubated in the dark at 30°C for 6 days. Percent kernel colonization (PKC), sporulation and aflatoxin were influenced by the maize genotypes (G), the location (“ear environment” or E) and the GxE interactions. Overall, low broad‐sense heritabilities were observed for PKC, sporulation and aflatoxin. PKC was significantly correlated with sporulation in all environments. Aflatoxin was positively correlated with colonization for two and with sporulation for all ear environments. Higher grain sulphur or magnesium in IBM was associated with less colonization or aflatoxin. Postharvest susceptibility of maize to aflatoxin is thus influenced by factors that are modulated by the ear environment. In a KSA, sporulation could be a proxy test for aflatoxin accumulation.  相似文献   

小鼠H-Y单克隆抗体ELISA检测方法的建立   总被引：2，自引：0，他引：2  

杭苏琴  刘为敏  牛树理  冯紫云 《中国兽医学报》2004,24(6):547-549

以纯系 BAL B/ c雄性小鼠脾细胞腹腔注射免疫同系雌性小鼠 9次 ,获得的抗血清经雌、雄鼠脾细胞吸收后用于精子细胞毒性试验 ,测得 H- Y抗血清效价为 1/ 16 0。选取免疫应答最好的雌鼠脾细胞与 SP2 / 0骨髓瘤细胞融合 ,用精子细胞毒性方法筛选效价较高的细胞株制备腹水 ,建立优化的 EL ISA反应条件。优化后的 EL ISA反应条件为 :抗原4℃过夜 ,加 H- Y抗血清 37℃反应 12 0 m in,加 HRP- Ig G 37℃反应 30 min,加 TMB 2 5℃ 30 min。优化后的 EL ISA与常规 EL ISA比较 ,可以明显降低阴性吸光值 ,检测灵敏度从 1/ 32 0上升为 1/ 12 80  相似文献   

鸡传染性法氏囊病间接ELISA诊断试剂盒的研制及初步应用   总被引：3，自引：0，他引：3  

马秀丽  崔言顺  张秀美  黄兵  崔治中 《中国兽医学报》2003,23(5):424-426

采用vero细胞增殖的IBDV抗原建立了间接ELISA，用于定量检测IBDV抗体。对该方法进行了标准化研究，确立了该方法的最佳工作条件。在此基础上研制了相应的诊断试剂盒，并对盒内各组分的性状、保存、质量控制以及诊断试剂盒的特异性、敏感性、可重复性、符合率、与国外同类产品的比较、保存期等进行了全面、详细的研究。结果表明，研制的试剂盒在-20℃保存至6个月时各项性能都很好。该试剂盒与进口试刺盒对同样血清样品检测，符合率为86．7％。间接ELISA试剂盒与琼扩试验的符合率为92，5％。该试刺盒可对大量血清样品进行检测，操作简单方便、结果特异性强、敏感性高、快速，更适合于大型鸡场IBD免疫抗体水平的监测及现地疫病诊断等需要。  相似文献   

蓝舌病灭活疫苗免疫羊ELISA和琼扩监测比较试验     

陈兴扶  范根成  马洪超  杨承谕  周勇  曹正惠  陈远坤  段金荣  冷光敏  郑贡诗 《中国动物检疫》1994,11(3):10-11

用19只绵羊（注苗前BTV琼扩和ELISA均为阴性）注射BTV灭活苗后7～139天的血清进行BTVELISA和琼扩平行试验，结果表明，注苗后7～30天11只试验丰ELISA阳性，注苗40天13只羊ELISA阳性，注苗90天以后全部试验羊只均为ELISA阳性，而琼扩试验则始终为阴性结果。  相似文献   

单克隆抗体ELISA检测犊牛粪便中冠状病毒抗原     

陈焕春  金梅林 《中国兽医杂志》1995,21(1):8-11

用两株单克隆抗体混合后包被ＥＬＬＩＳＡ微孔板，加牛冠状病毒抗原，加经白陶土处理过的兔抗牛冠状病毒免血清，再加上辣根氧化物酶标记的羊抗兔ＩｇＧ抗体，加底物质显色间接ＥＬＩＳＡ检测牛冠状病毒抗原获得成功。用此方法检测细胞培养的牛冠状病毒上清液，其敏感度高出血凝试验（ＨＡ）８倍，从武汉市附近３个奶牛场采集犊牛腹泻粪便１０５份，用单抗ＥＬＩＳＡ检测牛冠状病毒抗原，共检出阳性３６份，并与血凝及血凝抑制试验，  相似文献   

应用FA及PPA-ELISA技术对猪瘟的检测   总被引：3，自引：0，他引：3  

潘树德  何利昆  李学俭  马兴元 《动物医学进展》2003,24(5):114-116

用免疫荧光抗体诊断技术及单克隆抗体纯化酶联免疫吸附试验诊断技术对疑为猪瘟病毒感染猪进行了检测 ,重点阐述了 2种方法的技术原理和操作过程。通过用免疫荧光抗体诊断技术检测了 5份病料 ,其中有 2份为阳性 ,阳性率为 40 % ;用单克隆抗体纯化酶联免疫吸附试验诊断技术检测了猪瘟血清抗体 ,在 40头母猪血清样品中 ,猪瘟弱毒抗体效价 OD值较高 ,有 1 0 0 %的保护率 ,但是发现母猪群中有 1 0 %隐性猪瘟感染 ,其强毒抗体效价 OD值大于 0 .5,体内带有猪瘟病毒。结果及过程表明此两种诊断方法检测快速、鉴别准确、分辨率高  相似文献   

马传贫驴白细胞弱毒疫苗株跨膜蛋白主要免疫决定区基因的克隆与表达   总被引：3，自引：0，他引：3  

薛飞  贾斌  朱远茂  杨建德  王晓钧  相文华  赵立平  吕晓玲  沈荣显 《中国预防兽医学报》2003,25(5):321-325

从感染驴白细胞的马传贫驴白细胞弱毒疫苗株前病毒DNA中克隆了编码跨膜蛋白主要免疫决定区(TMIR)的基因，并在大肠杆菌中进行了表达。所表达的融合蛋白有一部分是可溶的，其氨基端带有6个组氨酸的标签，因此可以用固定化金属离子亲和层析法在非变性条件下进行纯化。在间接酶联免疫吸附试验(ELISA)和免疫印迹试验中，重组的TMIR蛋白可与马传贫阳性血清样品发生反应，而与健康马血清无任何反应。这表明该重组蛋白具有良好的抗原性和特异性，可用于马传贫弱毒疫苗株在体内外复制、接种马体内免疫应答及马传贫诊断的研究。  相似文献   

SMD残留检测的ELISA方法的建立和初步应用   总被引：12，自引：0，他引：12  

周新民  陈连颐  王捍东  王宗元 《畜牧与兽医》2003,35(10):8-11

用戊二醛法将SMD与载体蛋白BSA偶联 ,制备合成抗原SMD BSA作免疫原 ,同法合成包被抗原SMD OVA ,免疫健康家兔获得抗血清。分别用双向琼脂扩散试验和ELISA试验对抗血清进行定性定量测定 ,结果表明所获抗血清特异性针对SMD。用所制备的抗血清建立间接竞争ELISA方法。优化了ELISA的工作条件 ,方阵测定确定了包被抗原最佳浓度 (50 μg/mL) ,抗血清最佳稀释度 (1∶1 0 0 ) ,酶标抗体的最适工作稀释度 (1∶50 0 ) ,并建立了ELISA标准工作曲线。工作曲线表明在 1 0～ 2 0 0 0 μg/L浓度范围内呈良好的线性关系。该法检测底限为 63μg/L,低于国际规定残留限量 (1 0 0 μg/kg)和国内规定残留限量 (30 0 μg/kg)的要求。本法同时测定了回收率以及实际样品血清中的SMD的残留含量  相似文献   

Rotavirus infection in calves in Bangladesh     

S. A. Selim  K. M. S. Aziz  A. J. Sarker  H. Rahman 《Veterinary research communications》1991,15(4):327-333

Faecal samples from 434 calves under 1 year of age (307 diarrhoeal and 127 normal) were collected from three dairy farms and one village in selected areas of Bangladesh. The samples were tested by an enzyme-linked immunosorbent assay (ELISA) to detect the presence of rotavirus antigen. Of 402 dairy calves tested, 28 (7.0%) were positive, of which 21 (7.2%) were from diarrhoeic calves and 7 (6.3%) from non-diarrhoeic calves. Rotavirus infection varied from farm to farm (2.7–9.2%) and there was no positive response from any of the 32 village calves. Rotavirus was most commonly found in calves of 1 week of age or less (up to 22.2% in one group) but was not found in any calves later than 6 months of age. More than 80% of rotavirus-positive samples from diarrhoeic calves exhibited a titre of 128 or more (geometric mean 345±4.5), whereas non-diarrhoeal calves had titres less than or equal to 128 (geometric mean=29±1.9), suggesting that rotavirus infection in calves in Bangladesh was mostly associated with diarrhoea.  相似文献