不同直径胶体金结合霍乱毒素B亚单位的逆行轴浆转运及其应用

不同直径胶体金结合霍乱毒素Ｂ亚单位复合物（ＣＢ－Ａｕ）注射于大鼠不同部位，观察对神经元的标记效果。实验结果：（１）ＣＢ－Ａｕ较ＣＢ－ＨＲＰ注射靶区扩散范围小，经银加强后ＣＢ－Ａｕ呈黑色致密的圆颗粒。（２）肌肉注射以５ｎｍ和１０ｎｍＣＢ－Ａｕ对神经元的标记效果较好，１７ｎｍＣＢ－Ａｕ几乎难以标记神经元。在中枢神经系统，此三种直径ＣＢ－Ａｕ标记效果相似。（３）银加强标认神经元后可复合免疫细胞化学（ＩＣＣ）方法，双标记神经元的银颗粒与ＩＣＣ反应产物极易分辨；由此发现大鼠ｃａｌ－ｂｉｎｄｉｎ－Ｄ２８Ｋ阴性和阳性的红核脊髓投射神经元。（４）ＣＢ－Ａｕ滞留神经元内至少３５ｄ，故可行慢性实验。因此在比目鱼肌注射ＣＢ－Ａｕ的第５天切除该肌，３０ｄ后经银加强复合用ＣＧＲＰＩＣＣ仍能清晰分辨标认的神经元。结果表明，ＣＢ－Ａｕ为一很好的轴浆转运示踪剂尤适合复合ＩＣＣ的双标研究。

Expression of CTB-human Insulin(BA) Fusion Protein in Gynostemma Pentapyhllum Makino Callus Cells and Its Hypoglycemic Effect in Mice

The plant expression vector of choleratoxin B subunit（CTB）-human insulin（BA） fusion protein pBI121/（CTB-BA） was constructed first and then the Gynostemma Pentapyhllum Makino callus cell line that could express CTB-human insulin fusion protein was constructed and its hypoglycemic effect was evaluated in mice. The plant expression vector pBl 121/（CTB-BA） was digested with both BamI and SacI. Agrobacterium tumerfaciens strain LBA4404 was transformed with previously constructed recombinant plasmid pBI121/（CTB-BA） via the freeze thawing method, then CTB-BA gene was integrated to G Pentapyhllum Makino callus cells by co-culturing the cells with the transformed LBA4404 strain. The transformed G Pentapyhllum Makino callus cells were identified by DNA sequence assey and RT-PCR. The expressed product was identified by western-blot and its amount was tested by ELISA kit and its blood sugar decreasing effect was tested in mice. The sequences of synthetic CTB and human insulin genes（BA） were completely identical to those designed. Restriction map proved that the length of gene fragment in- serted into expression vector pBI121 was consistent with that expected. The sequence of genomic DNA of expressed product was completely identical to that designed. The result of RT-PCR was consistent with that expected. The expressed product showed a specific band with a relative molecular mass of 17000 by Western-blot. The human insulin expression amount was 6.03 μIU/mL according to the ELISA result. The animal test showed that only the G Pentapyhllum Makino callus cell line itself showed activity in decreasing the blood sugar of mice, however, the activity of the transformed G Pentapyhllum Makino callus cells was much higher, The plant expression vector pBI121/（CTB-BA） was constructed and expressed in the G Pentapyhllum Makino callus cells successfully for the first time. The trans- formed G Pentapyhllum Makino callus cells showed high activity in decreasing the blood sugar of mice. This study developed a new way for the development of oral administration insulin.

霍乱毒素或联合外周神经对再生视网膜节细胞c-Jun表达的研究

目的:观察成年金黄地鼠视神经近端微挤压断(MC)后,再生视网膜节细胞(RGCs)c-Jun的表达与再生的关系。方法:实验动物随机分为CTx组、SN+CTx组,每组5只。近端微挤压断视神经后,玻璃体内注射霍乱毒素(CTx)或联合植入小段坐骨神经分支(SN)。术后4W,用荧光金(FG)逆行标记和c-Jun免疫荧光组织化学双标法观察再生的RGCs和c-Jun的表达。结果:再生RGCs胞核内有c-Jun蛋白表达,CTx组表达c-Jun的再生RGCs为(317±61)个,约占其再生总数的89.9%;SN+CTx组c-Jun阳性再生的RGCs为(418±102)个,占再生总数的96.8%,两组相比差异有统计学意义(P<0.05)。结论:c-Jun表达可能与RGCs的再生有密切关系,霍乱毒素或联合外周神经可显著提高再生RGCs的c-Jun表达。

CB-Aβ抗体偶联物抑制痴呆小鼠脑内Aβ纤维斑块形成

目的研究CB-Aβ多肽抗体(IgG)是否能高效的进入痴呆小鼠脑内,发挥抑制Aβ纤维斑块形成的作用。方法用改良过碘酸钠法制备CB-IgG偶联物;鼻腔给予C57小鼠CB-IgG后用间接ELISA法测定脑内抗体量;给予C57小鼠抗体3 h后用间接ELISA测血清和脑区抗体量;5XFAD小鼠分为CB-IgG IN组,IgG IN组,IgG IV组,阳性对照组和阴性对照组,抗体干预14周后,双抗夹心ELISA检测脑内Aβ水平,免疫组化染色观察Aβ沉积和老年斑。结果鼻腔给予CB-IgG 0.3 h时在脑内即可检测到Aβ抗体的存在(P<0.05),3 h后达峰值(P<0.01);抗体给予3 h后,CB-IgG IN组海马区的抗体量高于IgG IN组和IgG IV组10倍以上(P<0.05),IgG IV组与IgG IN组脑内的抗体量接近;CB-IgG IN组小鼠脑内Aβ水平比阳性对照组显著降低(P<0.05);CB-IgG IN组海马和皮层区的老年斑面积与阳性对照组相比分别减少了80%以上(P<0.05)。结论鼻腔给予CB-IgG的方式,在提高抗体入脑量、抑制痴呆鼠脑内Aβ纤维斑块形成等方面均优于其他途径和措施。

加热霍乱类毒素的制备及其抗原性的研究

粗制霍乱肠毒素经60℃水浴,5分钟后其毒性丧失99％,抗原结合性保留87.5％。PAGE显示:毒素已成为大分子聚合物。将这种聚合物经口免疫小鼠,产生良好的肠道抗毒免疫和一定程度的血清抗体反应。

甲型H5N1禽流行性感冒病毒血凝素抗原和霍乱毒素B亚单位融合蛋白真核表达载体的构建与鉴定

目的构建甲型HSN1禽流行性感冒流感病毒血凝素（HA）抗原和霍乱毒素B亚单位（CTB）融合蛋白真核表达载体，并研究其在COS7细胞中的表达特性，及其在动物体内不同时间点诱导机体产生特异性抗体的情况。方法采用PCR技术分别克隆CTB基因和HA基因，并用BamHI酶切2个基因片段，在T4连接酶的作用下构建CTHA融合基因（CH基因）。双酶切后，将CH基因插入真核表达质粒pCI—neo中，构建甲型H5N1禽流感病毒融合蛋白真核表达载体（pCI—CH）。将pCICH质粒转染COS7细胞，利用Western印迹、十二烷基硫酸钠聚丙烯酰胺凝胶电泳（SD孓PAGE）检测HA抗原的表达；间接EI-ISA法检测免疫接种新西兰大白兔后其血清中HA抗原的特异性抗体效价，以及与H1N1、H9N1、H3N2和乙型流感病毒的交叉反应情况。结果pCl—CH真核表达载体（即核酸疫苗）构建成功，可在cos7细胞中高效表达，并能在大白兔体内诱导产生特异性抗pcI-cH抗体。核酸疫苗pC-CH特异性抗血清不仅可以与甲型HSNl流感病毒特异性结合（P／N〉2．1），而且可以与HINl、HgNl和H3N2毒株发生特异性反应；但该抗血清与乙型流感病毒无特异性反应。结论构建的甲型H5N1禽流感病毒核酸疫苗具有良好的免疫原性。